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DrawMap manual ver 2.2 Teemu Teeri 1991 First things first: The installation of DrawMap is described in the last part of this manual, Appendix F. Please note: This manual lacks all figures and tables. If you want to receive a printed manual and the latest update of DrawMap the shareware fee is $45. Please send check or money order to: Teemu Teeri Institute of Biotechnology P.O. Box 45 FIN-00014 University of Helsinki Finland Contents Chapter 1 Introduction What is DrawMap and what are plasmid maps How does DrawMap work Chapter 2 Using DrawMap - section by section Section 0 - Quit the program Section 1 - Draw a picture of the workfile plasmid Section 2 - Show restriction data from the workfile plasmid Section 3 - Get a new workfile Section 4 - Prepare a workfile from DNA sequence Section 5 - Edit the workfile Section 6 - Save the workfile Section 7 - Change the default drive and file directory Chapter 3 The EDIT section FILENAME; PLASMID NAME; SIZE; FORM; ARC DEFINITIONS; ARCS; GENES; SITES; SUPPRESSION LIST; PICTURE COMPONENTS; COMMENTS CLONING INSERT; DELETE; REPLACE; ROTATE; MIRROR IMAGE Chapter 4 The RESTRICTION DATA section Chapter 5 The DNA SEQUENCE section Chapter 6 The DRAW section Chapter 7 Customizing DrawMap The SETUP section COLORS; DEFAULT SETTINGS; PLOTTER DRIVERS PLOTTER DRIVERS Screen - circle only; Screen - full drawing; Screen - high resolution; BBC SE284 plotter; HPGL compatible plotter; Epson compatible matrix printer; LaserJet II compatible printer; PostScript printer; DeskJet printer Appendix A Editing and creating DNA size standard files (.STD files) Appendix B Editing and creating restriction enzyme files (.ENZ files) Appendix C Modifying the DMDISP.TXT file Appendix D The structure of the .MAP files Appendix E The DrawMap character set Appendix F Installation of DrawMap Chapter 1 Introduction What is DrawMap and what are plasmid maps Genetic engineering is a collection of techniques for a molecular geneticist to make specific combinations of genetic elements, analyze them and finally transfer them to the host where he wants to study their effects. Genes and other genetic elements consist of DNA, whose specific sequence of nucleotides gives the stretch of this macromolecule its biological meaning. DNA is also a substrate for various enzymes, with which it is possible to cleave, modify and join the molecules in a predetermined way and these biochemical reactions form the core of genetic engineering. The geneticist does not usually synthesize himself the molecules he combines, but takes use of the ability of the bacterial cells to do the job. The DNA sequence of interest is joined to other sequences that determine that the molecule will be replicated in the bacterial cell. These self replicating, usually circular DNA molecules are called plasmids. Many plasmids exist in natural isolates of bacteria and hold genes for resistance against specific antibiotics, for example. The molecules that are designed to be able to carry foreign sequences (inserts) are themselves combinations of sequences in natural plasmids and other sources, and are often called gene vectors. Besides plasmid vectors, the molecular geneticists also use vectors derived from bacteriophages, especially the lambda phage. Whereas plasmids are circular molecules, the lambda phage is linear (the ends, however, do meet during the life cycle of the phage). The sequence of nucleotide bases in a DNA molecule can be determined by biochemical methods. Another important way to document a DNA molecule is to show the physical map for recognition sites for DNA cleaving enzymes. These enzymes, called restriction enzymes due to their original biological role, can detect a specific sequence of bases on a DNA molecule and cleave the molecule, usually inside this recognition sequence. The length of the recognition sequence varies most often between 4 and 6 base pairs, determining also how often, on average, the enzyme will cut "random" DNA sequence. A wide collection of restriction enzymes with different recognition sites are known and commercially available. These enzymes form the tools to cut out predetermined pieces of the DNA molecule, which subsequently can be joined with another enzyme, DNA ligase. Therefore a map of the restriction enzyme recognition sites ("restriction sites") is very important to the user. The restriction sites form the physical frame for a plasmid map. In that frame, the geneticist can orient stretches of DNA he knows to have biological function, such as genes and gene expression control elements. The task of drawing a tidy plasmid map in scale is not excessively complicated but does require some time and effort of concentration. Therefore, the drawing of a proper and useful plasmid map is often delayed and a good map is not available during the period of work when it might be needed most. DrawMap is a program that produces tidy, in scale drawn plasmid maps for the everyday use of the genetic engineer and, in the end, the final maps for his publications. The program supports a variety of plotting devices ranging from matrix printers to pen plotters and laser printers. Maps can also be drawn on the computer video screen for a quick check of how the current construction will appear. How does DrawMap work Activities of the DrawMap program can be divided in two parts: 1) collecting, editing and maintaining the data describing the plasmid maps and 2) composing and drawing the map on the physical device chosen. As for drawing the maps by hand, the locations of the characteristics of the map are defined by their base pair coordinates. These characteristics are of three kind: 1) Point-like features on the map, typically restriction sites, called sites in the program. These are defined by their coordinates and can be given names. They are shown on the drawn map as marking lines perpendicular to the main circle and with their names and coordinates written also perpendicular to the main circle (Figure 1). There may be a large number of these sites and they often crowd in particular regions of the map. For this reason, their drawing is handled specially and they are spread in the crowded areas (see front cover). 2) Area-like features on the map, typically genes and also called genes in the program. These are defined by their end coordinates and can be given names as well. They are drawn as arcs inside the main circle and either or both ends of the arc can have an arrow head (Figure 2). The name is written inside the arc and follows its direction. Unlike for sites, the coordinates of the genes are not shown on the final map. The gene arc can also have zero length, which makes this a second point-like feature on the map, but presented in a different way from the sites. 3) The second type of area-like features on the map, typically indicating areas different in function (like genes or promoters) or origin (in a recombinant molecule), are called arcs in the program. The arcs form the main circle of the plasmid map. They are defined by more parameters than the genes: a) end coordinates b) arrowhead and its direction at the ends c) breadth of the arc d) number of pen strokes within the breadth, leading to appearances from open box, through a striped box, to a filled box (Figure 3). Arcs do not have names like the genes. In addition to the three map characteristics mentioned above, which can vary in number, the map has also a name and a total size (in base pairs). The final drawing has space for comments as well. All this data is entered and can be edited in the editing section of the program. They can be stored on a disk or diskette as a file for later retrieval. Thus, the user can have a collection of his plasmid maps on disk. In real life, plasmids come in families and some maps may have much in common. Therefore, the entering of the same parts for many maps is duplicated work and it is much simpler to edit an existing map to a new one. To facilitate this, the DrawMap program has capabilities of deleting parts of the plasmid map or, reversely inserting empty space to be filled in by new features or parts of other maps composed with the DrawMap program. These facilities simulate the way how new plasmids are constructed from preexisting ones in the laboratory with the methods of DNA cloning. In addition, it is always possible to edit, remove, or add sites, genes or arcs on the map one by one. The genes and arcs are always entered in the editing section. For sites, it is also possible to determine them directly from a DNA sequence. To be able to do that, the program needs to now a collection of restriction enzymes with their recognition sites. Such collections are provided with the program and they can be easily updated or created with a standard text editor. Besides drawing plasmid maps, the DrawMap program can also do restriction enzyme digestion simulations with the plasmids. This is related to the very common way of viewing isolated plasmid molecules by digesting them with some restriction enzymes and by visualizing the resulting fragments after separation by gel electrophoresis. The newly created or edited plasmid map can be drawn on screen at different resolutions (and speeds - inversely related to the resolution) to check the result while editing. Finally, the drawing can be directed to the hard copy device connected to the computer (a pen plotter or a matrix or laser printer). The plotter commands can also be stored in a file on the disk, from where they can be imported to many modern text editors to be included in a document as a figure. DrawMap has also a special batch feature that allows several maps to be drawn in succession automatically. Chapter 2 Using DrawMap - section by section The DrawMap program is divided into sections, which the user enters from the main menu (Figure 4). He can call the sections either by pressing the section number or a key corresponding to the highlighted character on the section name. Some sections are small and simple like the one that allows you to change the current drive and directory and others are large and complex like the editing section. In the following, we shall go through the different sections and show what the user can do in them and how to achieve it. Later chapters will describe in detail the more elaborate sections. The sections are covered here in the order of appearance on the menu. That, however, is not the order in which they are usually needed. General comments on keys: Nearly each section contains context sensitive help behind the function key F1. In some sections, a more general help window is initiated and in others, individual advice is provided on how to respond to a prompted question. Another key used repeatedly in a similar way is the ESC key. This key quits the current action, finishes compilations when needed, and returns the user back to the previous level. Logically, exit of the program from the main menu should take place with the ESC key. However, to prevent accidental exit, this does not take place and the user must use the Q key instead. Many times the user is asked a yes/no question. The answer is provided by hitting the Y or N key. Some questions take also RETURN for answer and use then the default choice. When more choices are offered, they are indicated with the question. CTRL-G and CTRL-V function as editing keys when text data is edited in different tables and boxes. CTRL-G deletes a character at the cursor position and CTRL-V inserts a space character (blank) at the cursor position pushing existing text simultaneously forward. Section 0 - Quit the program Purpose: Exit to DOS. Operation: Communication in the main menu window. Restrictions: None Notes: If the workfile has not been saved, the DrawMap program will prompt whether it will be OK to exit. Section 1 - Draw a picture of the workfile plasmid Purpose: DrawMap composes the plasmid map from the data in the workfile and sends the graphical representation to the physical device determined by the user. Operation: The main menu is left behind and a drawing menu is opened (Figure 5). The user picks up the physical device from the list by indicating its number. By pressing the B key, the batch function is activated. Instead of drawing the workfile map, DrawMap will draw all maps found in the current directory one after the other. Restrictions: 1) The workfile must represent a plasmid unless you have activated batch drawing. 2) The user's computer must be equipped with the hardware with which the indicated driver program is designed to function. Failure in this respect may lead to unpredictable results. In doubt, be sure that the workfile is saved first. Notes: This section is described in detail in chapter 6. Section 2 - Show restriction data from the workfile plasmid Purpose: The plasmid map files contain all the data to predict band patterns in gel electrophoresis of restriction enzyme digested plasmids. This section gives these predictions, either as fragment lists or as simulated gel images. Operation: The main menu is left behind. The user is prompted with questions concerning which enzymes to use in the digestions. Restrictions: The workfile must represent a plasmid (i.e., you cannot use a blank map). Notes: This section is described in detail in chapter 4. Section 3 - Get a new workfile Purpose: The plasmid map under construction or which is otherwise worked with is called the workfile plasmid. In this section the user can pick up a new map saved on the disk or, alternatively, start to construct a new map. Operation: Communication takes place in the main menu window. DrawMap prompts for the name of the new workfile. List of all .MAP files in the current directory is shown when the help key F1 is hit. You can load a map file also from another directory by providing a path, e.g. A:\MAPS\PBR322. Restrictions: The entered reply must be a legal DOS file name. If you specify a path, the file must also exist. Notes: Taking a new workfile automatically abandons the previous workfile. If it had not been saved, the DrawMap program will comment on the situation. You can withdraw from picking a new workfile by entering a blank line. If the entered filename corresponds to an existing file, that one is retrieved as the workfile. If the file does not exist, the work file represents a blank plasmid map. The plasmid map files created by DrawMap have usually .MAP as their extension. This default extension does not have to be entered. If the help key F1 is hit after typing in characters, not all .MAP files in the directory are shown but only those whose filename will match for their beginning the entered characters. Section 4 - Prepare a workfile from DNA sequence Purpose: Restriction sites on a DNA sequence can be searched in this section in order to be used as a basis of a new plasmid map. Operation: The main menu is left behind. The user is prompted with questions concerning where to find the data for the DNA sequence and the restriction enzyme recognition sites (the enzyme data can also be entered from the keyboard). Restrictions: The DNA sequence must exist on disk as an ASCII file, from which only the letters A, C, G, and T (either upper or lower case) are extracted. Notes: This section is described in detail in chapter 5. Section 5 - Edit the workfile Purpose: This section collects all the necessary data to build a map. Editing of existing data is also straightforward and DNA cloning can be simulated. Operation: The main menu is left behind. The user moves around with arrow keys in a table of data which he can edit. Notes: This section is described in detail in chapter 3. Section 6 - Save the workfile Purpose: The workfile is saved in the current directory. Operation: Communication in the main menu window. Restrictions: The workfile must represent a plasmid (i.e., you can not save a blank map). Notes: If a file with the same name as the workfile already exists in the current directory, the user is prompted of whether it should be written over. Usually the pre-existing file represents a previous version of the same plasmid map. The previous version is not destroyed. You can find it under the name LASTMAP.BAK in your map directory. Only after the next saving operation the data will be lost. LASTMAP.BAK always contains the data of the latest overwritten .MAP file. This makes it possible to regret your savings. Section 7 - Change the default drive and file directory Purpose: Changes the disk drive and directory from where saved plasmids maps are retrieved and where they are filed when saving. Operation: Communication in the main menu window. DrawMap prompts for new (drive and) directory. Restrictions: Entered reply must correspond to an existing (drive and) directory. Notes: If you start DrawMap by entering a directory name as a program parameter (by typing at the DOS prompt e.g. DRAWMAP A:\MAPS), the program will change into that directory while starting. For different users, it is practical to have personal DOS batch files that will take DrawMap directly into the correct personal directory (see appendix E). Chapter 3 The EDIT section This is the section of the DrawMap program with which the user can build a new map or edit one built earlier. It also allows the user to insert parts of other maps into the plasmid or replace parts with those of other maps, much in a similar way as plasmid construction is made by DNA cloning techniques in the laboratory. In the edit section, the data forming the plasmid map is presented as a series of tables. The user moves the cursor into the tables and enters or edits the data there. Special keys move the cursor and edit the data. These keys are collected in table I and appear also on the screen when the help key F1 is pressed. Each time the cursor exits a data table (which may contain only one row of data), the entered data is checked. If it cannot be interpreted in a sensible way, the cursor moves back to the erroneous item. Also, data in some tables are compiled when the cursor exits the table, e.g. restriction enzyme sites are ordered in ascending order by their position coordinate. Many data tables allow a long list of data items to be entered. In those tables, the empty rows are hidden and more space is opened only when needed. The whole editing screen, which scrolls up and down when you move in it, is shown in figure 6. FILENAME This holds the DOS filename for the plasmid map. The map will be saved on the disk as a file under this filename. Therefore, the text entered must follow the DOS file name rules, i.e. contain up to eight characters, a period, and up to three characters in the extension part. Using upper or lower case letters here make no difference. If the period is left out, the DrawMap program will add .MAP in the name. You can type in other extensions if you wish, but it is practical to use the suggested extension. Since the program knows to expect it also elsewhere and you will save some typing. If you want to build a new map based on an old one, be sure to change the filename in this table. Otherwise, when saving the map, it will replace the previous one on the disk. PLASMID NAME This is the name of the plasmid that is written in the center of the map. You can enter any characters, including spaces and special graphic characters here and they will appear as such on the plasmid name. Please note that the standard IBM character set has been modified in DrawMap to include important characters such as the lower case lambda (■). However, these modified characters appear on screen as unmodified. They are treated in a special way only by the drawing procedures. The full available character set is described in appendix D. SIZE Here you can enter the size of a new plasmid. When editing an existing map, you can not change the size by entering a new value here. Instead, the deletion and insertion functions in the cloning menu must be used. FORM The form of the plasmid is either circular or linear (see Figure 7). Internally the map is presented as a circle independent of the form which means e.g., that in both cases the coordinates zero and size refer to the same point and not to the opposite ends of the linear form. The form is changed by hitting the key L or C when the cursor is on the appropriate row. ARC DEFINITIONS This table holds reference data on how different areas on the plasmid main circle are drawn. Each arc definition has a number that is referred to in the following table ARCS. Different types of arcs are formed by varying the three parameters: thickness, lines and pen. The thickness or breadth uses as a unit the radius of the circular map. Lines tells you how many equally spaced arcs are drawn within the thickness. By determining two arcs, an open box type arc is drawn and by determining many, a filled black box is drawn. Between these two extremes, you can get striped arcs (see Figure 3). The parameter pen is very device dependent. On xy-plotters using real pens, it refers to the pen number on the pen rack that the user fills according to his choice. On matrix printers or lasers it refers to the thickness of the line (but only in high resolution), and on screen devices, it refers to the color (if available). In addition, pen number 0 is treated differently in different devices. On xy-plotters it logically means no pen but on matrix printers or lasers (only high resolution again) it means extra thin lines (e.g., for miniature maps). Therefore, if you want to leave part of the map blank (Figure 8), do not define an arc type with pen=0 but lines=0. Thickness=0, on the other hand, leads to a simple, single stroke line. The program defines four predefined arc types: single, heavy, double and broad double, which however can be modified freely. The default definitions serve as starting points for users own definitions which may amount up to 20 different. To change the predefined types permanently, see appendix C. Still one word about pens. Genes and sites are also drawn by a pen but they do not have a pen number definition in their tables. Instead, genes are drawn with the pen of arc definition number 2 and sites (as well as all the rest) with the pen of arc definition number 1. Normally you don't need to be concerned about this. Only when you want to play with different pens, it is important to know this. ARCS Varying arcs on the main circle of the plasmid gives character and a clarified appearance for the map. Arcs are defined by their startpoint, endpoint and kind - the latter referring to the arc definitions described above. In addition, the borderline between two arcs can be an arrowhead, either to the left (counterclockwise) or to the right (clockwise). These are added by using the > and < keys and can be removed by pressing CTRL-A. The arrowhead is always drawn on the arc that has larger thickness, defined in the arc definition table. Normally the tip of the arrowhead is at the coordinate of the arc junction, but on short arcs (appearing as triangles) it pushes towards the arrow direction. Arcs are added to the arcs table freely. It is important to know how they are compiled when the cursor leaves the table. DrawMap program first creates a basic map with arc type 1 all over. On top of this, it adds first the arc defined on the first row of the table, then from the second row and so on, discarding older definitions from areas covered by new ones. This means that the arc table can change a lot when the user knows how to take advantage of this compilation. Clearing the arc table is done simply by adding a full length definition on the last line and exiting the table. The length of each arc must be at least one base pair. An arc with the same startpoint and endpoint coordinate is interpreted to mean a full round arc (which also cancels all previous definitions due to the way of compilation). Note that with genes, exactly the opposite interpretation is done. GENES Genes are defined by entering their startpoint, endpoint and name (which may be blank). Either end can have an arrowhead that has fixed direction: outward from the gene. The arrowhead is added to either end by pressing the < or > key while the cursor is on the end coordinate and removed by pressing CTRL-A. In the final map drawing, the name of each gene is written along the gene arrow and centered in respect to it. For the characters to be in a readable orientation, the name is written clockwise in the upper half of the map and counterclockwise in the lower. The direction is determined by the midpoint of the gene and is shown as a plus or minus sign in the column D (for direction). In special cases you can force the direction by entering a + or - in this column. The program does the midpoint calculation only when the column is left blank (an exception to this is when you have done cloning). You can redo the calculation by entering a space in column D and moving to another row. A gene with startpoint and endpoint equal is considered to have a zero length. SITES Sites are typically recognition sites for restriction endonucleases. They are considered point-like (although the recognition sites really span 4-6 base pairs) and are defined by their coordinate and name. The last column contains information for the RESTRICTION DATA section only: sites marked as enzymes are cut in a digestion simulation (see that section). All sites are enzymes by default and can be changed to markers by pressing CTRL-T at the appropriate site row. A practical feature while entering sites is that if the name is left blank, it is copied from the previous row. Therefore, you can enter all sites with same names sequentially by typing only their coordinates and rely on their reordering after exiting the table. However, this feature makes using blank site names difficult. You can enter them by first opening extra space in the table with the RETURN key and typing in the enzyme separately of others. Upon exiting of the table the blank enzymes will be ordered properly. However they are unstable: if you pass through the table, they will get names of their predecessors on the table. To obtain "stable" blank site names, you should use the non-printable character with code 255 (see appendix E). SUPPRESSION LIST You can suppress the drawing of particular map components by changing their status on the list by pressing CTRL-S. For example, if the coordinates are not accurate, it may be better not to show them at all. The map and the comments can also be framed - an option that you can choose here. PICTURE COMPONENTS The appearance of the map can be modified by modifying the size parameters for the various parts of the map. E.g., crowded areas for genes are not resolved in a similar fashion than for sites so that the only means to clarify them is to reduce the character size. Note that you can also change the shape of the characters (Figure 9). All units here are again parts of the map radius. The default values to give "standard" maps are shown on the right column and pressing CTRL-D here retains that value instead of clearing the row. The last parameter, magnification, is very useful. The default magnification (1.0) allows space for full length site names (20 characters) and the map remains often unnecessarily small. For each map, the program calculates the maximum magnification that still retains all features within the borders of the picture. However, this is only a clue and higher magnifications are allowed but will lead to clipping off of parts of the map. COMMENTS Finally, the map has ten rows of space for comments that of course are completely free in format. As with other default settings in these tables, the comment field can hold as a default, e.g. your address. See appendix C to define the defaults used for all new maps. CLONING Filling in of the tables described above takes place when a new plasmid map is constructed from scratch. In real laboratory life, new plasmids are constructed from preexisting ones by recombining fragments of them. The DrawMap program can simulate this kind of DNA cloning. The cloning section is entered from the editing section by pressing the F2 key. The actual cloning functions are INSERT, DELETE and REPLACE. The functions ROTATE and MIRROR IMAGE found in this section as well, do not change the content of the map. A cloning function is chosen by pressing the appropriate number key. Before the cloning step is finished (i.e., during the entry of the relevant coordinates), pressing ESC will lead to cancellation of what was started. The operation of the cloning functions is the following: INSERT With this function it is possible to insert a foreign segment at a particular coordinate on the map. If that coordinate contains a site, the site will appear at both ends of the insert. After the entry of the insertion coordinate, the user will be asked for the source of the insert. Entering a blank line here inserts a blank, featureless region on the map the length of which is asked next. Alternatively, entering the name for an existing plasmid map, the insert will be taken from that plasmid. (If the source map file is not in the current directory, drive and directory data can precede the file name. The extension .MAP can be left out, e.g. C:\MAPS\PBR322). Again, coordinates to define the insert are asked. It is important to enter first the left coordinate (5' for the geneticist) and then the right (3') coordinate. When the origin (coordinate zero) is included in the map, the startpoint coordinate will be larger than the endpoint coordinate. If the startpoint and endpoint coordinates are equal, the whole source plasmid is inserted into the workfile plasmid. The orientation of the insert is defined next. Pressing + (or RETURN) inserts the fragment in the same orientation as it is in the source map and pressing - inserts it in the reverse orientation. The INSERT function joins the ends of the insert to the insertion coordinate on the current (workfile) plasmid. If the joining point contains the same site (by name) on both maps, they are fused to one, exactly like in DNA ligation. If the two sites are different, they still are joined, but a new name for the combined site is asked for. If you enter a blank line for the name, the combined site is discarded. DELETE The function DELETE is the reverse of the function INSERT. You need to provide the startpoint and endpoint coordinates and everything between these is removed from the map. The ends are joined and if they contain the same site, that is retained at the joining point. Again, if both ends do contain a site but they are different, a new name for the combined site is asked. REPLACE REPLACE is a combination of DELETE and INSERT. The segment of the current plasmid to be removed is defined by its startpoint and endpoint coordinates, as when using DELETE. The source of the insert is entered exactly the same way as when using the INSERT function. Also, sites at the joints are treated as in INSERT and DELETE. ROTATE ROTATE is a function with which you can rotate the map into a new orientation. The program will ask which coordinate will become the new origin (coordinate 0). After rotating, all coordinates have new values. MIRROR IMAGE MIRROR IMAGE function inverts the map. The axis of mirroring is defined by entering a map coordinate. After each cloning function, the user still remains at the cloning window and can use any of the functions again. You return to the EDIT section by pressing ESC. Similarly, the DrawMap MENU is reached from the EDIT section by pressing ESC. The current table is exited automatically before the EDIT section is left behind. Chapter 4 The RESTRICTION DATA section The point-like features called sites on the plasmid map are typically recognition sites for restriction endonucleases, specific enzymes that cut the DNA molecule at their recognition site. The fragments produced can be separated according to their size by using gel electrophoresis and visualized by staining with particular dyes. This kind of fragment "fingerprint" is a routine way to identify a preparation of plasmid molecules. The RESTRICTION DATA section calculates an ordered list of the fragments produced by digestion with one or several restriction enzymes. It can also simulate gel electrophoresis and show on screen a simulated image of the electrophoretic analysis. This allows easy comparison of the expected and actual electrophoretic results. The section works by presenting questions to which the user answers. The first question is whether the fragment list will be sent to the parallel printer attached to the computer (in LPT1). Allowable answers are Y for yes, N for no and F for printing the list of the fragments but omitting the startpoint and endpoint data for each of them. Next you enter the names of the enzymes in the simulated digestion (corresponding to the sites on the map), each on a separate row, i.e. separated by pressing the RETURN key. When all enzymes are entered, press RETURN once more and the ordered list of the fragments produced is shown. It is important to know how the entered enzymes and the sites on the map are matched. The program considers that the enzyme cuts the site if the site contains the entered enzyme name as a part of it. In addition to the normal one-to-one match, this means for example that the enzyme 'Ava1' will cut also the site 'Sma1 Ava1'. However, you must be careful since 'Hind' cuts both 'Hind3' and 'Hind2', which perhaps was not the purpose. The entered enzyme name can have trailing spaces. Therefore, if you enter 'Cla1 ', this cuts the site 'Cla1' but not 'Cla1 (dam)'. From the above it is clear that the spelling of the entered enzyme name must exactly match the spelling of the sites and, also, that using upper or lower case letters now does make a difference. To make all this easier, the F2 key will list the different sites on the map with their exact spelling. Beside the site name the number of its occurrence on the map is shown and, also, the sites that were recognized in the last digestion are highlighted. After calculating the fragment list, the program waits for new enzymes for the next digestion. Before going forward you can inspect the gel simulation by pressing the F3 key. The gel simulation plots the fragments on the screen according to the logarithms of their sizes (Figure 10). This is a reasonably good simulation for a real gel. The smallest fragment visible at the lower edge of the monitor is about 800 bp in size and the still smaller ones run downwards out of the monitor. By pressing the UP ARROW key you can compress the gel and see the smallest fragments and correspondingly by pressing the DOWN ARROW key you can stretch the gel and separate better the large fragments from each other. This effectively simulates varying the concentration of the gel matrix or run length of the electrophoresis. Beside the digestion pattern of your plasmid DNA, a DNA size standard is shown. You can change the size standard by pressing the F2 key. The size standards are held on disk as data files. If you want to pick one of those, answer F to the first question. A list of available standard files will appear on the screen and you pick one by entering its name. (The extension .STD can be left out.) On entering the RESTRICTION DATA section, DrawMap automatically picks a predefined standard file. You can change this in the SETUP section. Alternatively, you can enter the sizes of the fragments in the standard from the keyboard. To choose this, answer K to the first question. You can first give the standard a name that will appear on the gel simulation (max 20 characters). Next the fragments in the standard are entered in base pairs (in any order) and finally, after entering a blank line to indicate that all fragments are entered, you can give the list a file name (in DOS format) if you want to save it on disk for later use. Chapter 5 The DNA SEQUENCE section The EDIT section allowed the user to enter restriction enzyme cut sites by their coordinates and names. This section allows a very different but useful way to enter the sites, directly from a previously recorded DNA sequence. (This section may be helpful also in the primary analysis of DNA sequences.) The sequence must be on the computer disk or diskette as a file consisting of ASCII characters. Only the characters A, C, G and T (as well as N, and X for unknown bases), either in upper or lower case, are recorded and others are discarded. The other file needed is the file for restriction enzymes and their cut sites. The DrawMap program package contains two such files, the files ALL.ENZ containing commercially available restriction enzymes and their recognition sites and 6BASE.ENZ containing restriction enzymes with at least six base pairs long recognition sequences. These files are text files and they can be modified and edited with any standard word processing program. (For details, see appendix B.) Unlike the DNA sequence, the list of restriction enzymes can also be entered by hand from the keyboard. This is practical when only a few enzymes need to be scanned. The entered list can also be saved on disk for later use. A site for an enzyme in the DNA sequence is scored when the recognition site of the enzyme matches, base pair by base pair, a stretch in the DNA sequence. The match is tried simultaneously also on the other strand of the DNA molecule (not recorded but implicit by the biochemical structure of DNA), unless this feature is disabled (see later). The site coordinate will be at the first base pair matching the enzyme's recognition sequence. Note that this is not connected to the actual cut site that varies depending on the enzyme and is not known for all of them. If there was no workfile map when this section was entered, one equal in size to the length of the recorded DNA sequence will be created. However, if a workfile exists, the new enzymes found in this section will be put among the previously existing ones. The workfile plasmid should not be smaller than the length of the recorded sequence! If you intend to "clone" (insert) the recorded DNA sequence into a preexisting plasmid, you should perform the following functions first in the EDIT section cloning menu: 1. Choose the site of insertion and rotate it to the desired location, usually to point zero. The first base pair of the recorded DNA sequence will have coordinate 1. 2. If necessary, mirror image the map to get it in the desired orientation with respect to the DNA sequence. The recorded sequence cannot be mirrored, but you can mirror again the end result. 3. Insert, at the chosen site of insertion, blank space corresponding in size to the length of the DNA sequence. Perhaps you also want to define its arc type and insert a gene arrow in it. See EDIT section for details. Now you have arranged blank space in your map, starting from coordinate 1, and the site coordinates read from the DNA sequence will fall in their right places. The DNA SEQUENCE section has two parts. The first part is question-answer oriented and its purpose is to locate and read the sequence and enzyme files. The second part is a list of all enzymes from the enzyme file together with indication of how many sites was found. These are usually far too many to be all included in the map and part of the enzymes must be discarded. This is done by moving around in the table with the arrow keys and doing the decisions with special keys. Behind the help key F1 is information about the special keys that can be used (see also Table II) as well as on the color coding used in the enzyme table. The first part starts by prompting for the name of the DNA sequence file. If you use a DNA analysis software that produces DNA sequence files with a standard file name, you can make DrawMap to suggest this file name automatically (see the SETUP section). The file name must be in DOS format and it may contain drive and directory specifications. You will be returned to this question until you enter a name for an existing file or press ESC to return back to the main menu. When the program locates the sequence file it reads it into the memory. The maximum length of the sequence depends on how much free memory you have at the time and can be increased by removing any memory resident programs. Only the characters corresponding to bases in the biochemical structure of DNA are recorded, as well as two characters that can be used to indicate unknown bases (that is A, C, G, T, N and X - either upper or lower case). There is one functional exception to this: DrawMap stops to consider the line that contains the first encountered non-base character (not counting numbers or blanks). That string might be a name for the sequence. You will be asked whether to skip it when reading the bases (then it is a name and will be recorded as plasmid name if there doesn't exist one already) or not (in which case the A's, C's, G's, T's, N's and X's are extracted from it!). When reading is done, a short statistics is shown. In addition to the number of base pairs recorded, the number of blanks and digits encountered are show. Also, and very importantly, the number of other characters is shown and if this is not zero, the first forty are displayed. This list should be empty and if it is not, it probably means that your DNA sequence file was not what you thought it was. It may have contained also amino acid sequence data or it may have been a completely unrelated file. Note that in the string of other characters there are no A's, C's, G's, T's, N's or X's - they have bee extracted into the recorded sequence. When other characters are encountered, the program asks whether you would start over. Usually you should. Next step is the reading in of the enzyme file. If you have the appropriate enzyme file on disk, press F in response to the next question and enter the enzyme name. The list of the enzyme files found in the \DRAWMAP directory is shown at the upper right corner and again you can customize the program to offer you a choice (see SETUP section). To access other enzyme files than those listed, you must include (drive and) directory data (all in DOS format, of course). Alternatively, you can enter the enzyme list from the keyboard. You will be first asked for a name for the enzyme and then its recognition site (upper and lower case don't make difference). Many enzymes have several possibilities for a match at a particular position. These are coded by other alphabetical characters than A, C, G and T (See table III) and you will get the list on screen by pressing the help key F1. Note that all non-listed characters behave as the character N and will match anything (type carefully!). The list is ended by entering a blank line for the recognition sequence. After that, you have a chance to save the list on disk with a file name of your choice (but in DOS format). If the period in the file name is left out, the default extension .ENZ will be added. This is a practical way to enter short enzyme lists, but for longer ones, see appendix B. Before the actual scanning you will be asked whether both strands on the DNA sequence are scanned. This is a natural thing to do for restriction enzymes (but, however, makes a difference only in those few enzymes that do not have palindromic recognition sites). The real meaning of the question is to allow efficient "misuse" of the section. The "enzymes" do not necessarily have to be restriction enzymes and the "recognition sequences" what they were originally meant to be. You can scan any kind of sequence matches (including mismatches, see table III) on the recorded DNA sequence. If you scan for example for ribosome binding sites or polyadenylation sites, only one strand (the recorded strand) is meaningful to scan and in such a case you answer NO to the last question. What happens next is that the screen changes and you start to get an expanding list of the enzymes entered in the previous part. Each enzyme will have a number attached to its left - that indicates the number of sites found on the DNA sequence. There is also color coding: the enzymes with no sites appear blue and others green. (The color coding can be altered in the SETUP section to fit your taste and screen.) When the list is through, the bottom of the screen shows you the total number of found sites, which often exceeds the upper limit of 150 allowed sites. The last enzyme will be highlighted and the cursor is at the name. If you hit the arrow keys, the cursor will move to another site. If you hit the - key, it will turn to red (or magenta) and will become "unchosen". If you hit the + key, it will appear green (or blue) again. The SPACE BAR key will toggle between these two. This is how you choose and unchoose your enzymes. When you unchoose an enzyme with found sites, you can see the total number of sites change. If you unchoose an enzyme with no sites, the total number of sites does not change of course, but the operation still has meaning. The program lists in the comment field of the map those enzymes that do not cut, but only those that are chosen. (If the comment field already has text, the enzymes will be put in areas of blank space. Note also that there is no warning if all intended enzyme names do not fit in the free space of the comment field.) Besides moving around with the cursor keys and choosing or unchoosing individual sites, you can also categorically unchoose all sites with more than a particular number of sites by pressing a numerical key (See table II for all the alternatives). Finally, when you are ready, press ESC to return to the main menu. Be patient, the final processing of the wanted and unwanted sites takes a short while. Chapter 6 The DRAW section Entering this section brings you to a list of physical plotting devices which is much of your own product when you chose the devices in the SETUP section. You pick the one you want by pressing the appropriate number key and what happens next depends again on what you set up yourself. The descriptions of the different devices supported and how they are installed are found in the SETUP section. Below the list of the files there is the code B for batch. By hitting this key, an indicator will switch on at the upper left corner but nothing else happens. (You can toggle the indicator on and off with the B key.) What batch does is that instead of drawing the workfile plasmid map, the DrawMap program will draw all the maps sequentially in the current directory. The current directory is shown at the bottom of the screen and can be changed in the main menu. This is very practical when you need to produce a series of maps since normally you would have to change the workfile between the maps. After batch drawing is started, no user intervention is needed and tens of maps can be produced automatically. Batch drawing can be used with any physical device that itself does not need user action (like changing of paper) between the drawing of successive pages. Also, for the fun, drawing on screen can be run in batch. Each map is shown for five seconds before the next is taken under processing. Error handling is different from normal when maps are drawn in batch. Normally error messages are displayed on screen. When BATCH is active, a special file named DMBATCH.LOG is created in the directory where the map files to be processed are. That contains a list of all the map files found, together with any communication directed to the user. It is a good practice to check this file after each run with BATCH on. The error messages may be informative if you think that some maps are missing. Note that when you draw maps in batch, only those files with the extension .MAP will be recognized. Please refer to the SETUP section to see the description of each of the devices supported. Chapter 7 Customizing DrawMap In the EDIT section it was described how the picture component dimensions such as character size, length of the site mark, magnification can be modified to obtain more appealing maps or special effects. It is possible to incorporate modified values in the DrawMap system as defaults that are used for each new map. This is done by modifying the file which is used to form the editing screen. This file (DMDISP.TXT) is a text file that can be edited with a standard word processor. Besides modifying the picture component dimensions, you can incorporate data beforehand in the tables, in order to permanently define new arc type definitions or alter the existing ones, include your name and address to the comment box, or to determine which map components are drawn (the suppression list). These modifications will affect every new map composed, the old ones will not be touched. Also some other files used by the DrawMap program are plain text files in order to make their customization easy. The list of restriction enzymes with their recognition sites (the .ENZ files) and DNA size standards for the gel simulation (the .STD files) are such. In fact, the .MAP files themselves are text files, too. It is not necessary to edit the .MAP files directly but it indeed is possible and their readable structure makes it easy for a foreign program to use them. The structures and instructions for the editing of these text files are described in appendixes A-D. The SETUP section In addition to the possibility of editing the text files, the DrawMap program has within it a section to customize the screen colors, some default file and directory names and, very importantly, the list of plotter devices to draw the plasmid maps. The SETUP section is not entered in a similar way as the other sections. When starting the program, type DRAWMAP SETUP The SETUP MENU is shown in Figure 11. You move the arrow to point the item you want to customize and hit RETURN. COLORS In the color customization a cartoon version of each DrawMap screen appears, drawn in the present colors. You move the cursor with the arrow keys and when you want to change the color of a particular piece of text under the cursor, press the F1 key. On top of the screen, a box with all the possible color combinations will appear, the cursor blinking at the one corresponding to what are the present colors and what you wanted to change. Again, use the arrow keys to move the cursor on the color combination you want and hit RETURN to change the color on the DrawMap screen. If you are not satisfied, repeat the sequence. Sometimes, when the colors are badly off the capabilities of your monitor (e.g., when you use a monochrome monitor), you may not see all the text to be seen since some text is of the same intensity as the background. By pressing the F2 key, you can remove all colors and be sure to see everything that will need customization. Note that some colors on the screen, especially backgrounds, go in groups so that by changing the background of a particular item, also backgrounds of other parts will be changed. DEFAULT SETTINGS You can tell DrawMap in advance into which directory it should switch into when starting. (This corresponds to changing of the drive and directory from the main menu. If you give the drive and directory as a program parameter, it overrides the default setting described here.) Similarly, you can make the program to pick or suggest a standard file for the reading of DNA sequence, restriction enzymes or DNA size standard. This is done by typing in the appropriate directories or file names on the default settings screen (Figure 12). PLOTTER DRIVERS When you install the DrawMap in your computer or when you get new plotting equipment, you must define the plotter drivers. You can have up to nine plotter drivers assigned from which to choose (physically different devices or same devices with different parameters). If you need something in excess to this, modify the plotter drivers temporarily, for that run only, by exiting the SETUP MENU with the ESC key instead of the F2 key after making the changes. (F2 saves the setting on disk but ESC doesn't.) When you start to modify your plotter drivers, the first screen shows the preexisting list of choices. Initially it will contain only two different graphics screen drivers (Figure 13). You can remove assigned drivers from the list with the F1 key. To assign a new one, move the cursor to a free row and press RETURN. The screen will change into a list of the different plotter drivers programmed in the DrawMap Program (Figure 14). They will be described in detail later in this chapter. Again, by moving the cursor with the arrow keys and pressing RETURN, you choose the device you intend to assign and the screen changes. On the last screen (Figure 15), you define the communication parameters etc. Note that not all plotters will have the full list of parameters depicted in Figure 15. E.g. for the screen drivers the communication port ("device") need not to be specified, nor the baud rate when you have chosen a parallel port. The parameters not needed will simply not appear on the screen. The first row is a description of the plotter device and it initially shows what was on the device list (Figure 14). This description will appear on the DRAWING MENU (Figure 5) and if you choose several versions of the same plotter (e.g. with different resolutions or communication ports), it is very important that you edit the description to show the differences on the DRAWING MENU. Also, instead of retaining something like "HPGL compatible plotter", it might be more helpful for all users to type in the name of the actual plotter you have. The device box determines at which communications port the plotter is plugged in. The program supports two serial ports (COM1 and COM2) and three parallel ports (LPT1, LPT2 and LPT3). If you choose the serial port, you must also define the baud rate, the parity, and the number of data and stop bits. The format of this definition is the same as in the DOS command MODE COM (please consult your DOS manual for details). The destiny of the data need not to be either of the communications ports. It can also be a file on disk (or the NUL device, i.e. nowhere - this has mostly meaning for testing the program). If the entered text in the device box doesn't match to any of the ports or the NUL device, it is taken as a file name. The file name is checked for proper DOS format only when it is used, so that you can leave the box also blank in order to direct the data to a file the name of which is asked later when it is needed. The directing of plotting data into a file is meaningful when you use the HPGL or PostScript drivers. Many word processing programs can pick up pictures composed by using these standard plotter languages and therefore you can incorporate maps drawn with the DrawMap program into your documents. This possibility has been used extensively in the manual you are now reading. You can direct data for the matrix and laser printers into a file as well, but they will be more difficult to use and, do remember, very large (up to one MB). The directioning of data into a file can also be used as a universal device. If you enter, run time, as a file name any of the port names or the null device mentioned above (i.e. COM1, LPT1 etc.), the destiny will be the port or null device designed. Note that the baud rate of the COM ports will then be whatever it was set to be earlier. The model box is something which is very specific to each plotter and appears only when there are different choices. For HPGL plotters it refers to the orientation of the paper (portrait or landscape) and you should choose the one that matches your plotter. For the raster devices (matrix and laser printers) it means resolution. Maps with coarser resolution are naturally faster to produce and you may want to include them to make fast draft maps. You choose the "model" by hitting a number key and the box will automatically show the choice in readable language. Last on the list, you can order DrawMap to pause and wait for a key stroke before it starts sending the data. Whether you need this, depends on your particular arrangement of things. Especially with xy-plotters (pen plotters) it may be wise to stop to check that everything is ready before starting the drawing. When you exit this last screen, you will find the new plotter incorporated on your plotter list. You can go on and assign new plotters (or edit the parameters of the ones already assigned) or retreat from the SETUP section by pressing repeatedly the ESC key. Note that the changes made in the SETUP section are saved only when you exit the SETUP MENU with the F2 key. If you exit with ESC, they will affect only the current run of DrawMap. PLOTTER DRIVERS The current version 2.1 of DrawMap contains nine different plotter drivers. Three correspond to a graphics screen at different resolutions (and speeds of use). All the screen drivers can be used with the CGA, EGA, VGA and Hercules screens. The drivers will be described in detail here. Screen - circle only This is the coarsest resolution screen driver but fastest to use. It draws only the arcs, genes and the site marks but leaves away all text (Figure 16). If the monitor can use colors at the 320 x 200 resolution, use of different pens is shown as different colors. Pen number 0 is not visible. The main use is to check quickly the overall composition of the map. Screen - full drawing This screen driver draws the whole map on screen with comments and texts as they would appear in the final form (Figure 17). The highest available resolution of the monitor is chosen and if this allows colors they are used as with the previous driver. The high resolution screens (like the EGA and VGA) allow resolving of the individual characters but with the CGA monitor only a coarse general image can be obtained. In all cases this driver is very useful in checking the actual positions of gene names etc. on the map. Screen - high resolution The resolution of this screen driver is 640 x 874 pixels independent of the monitor used. Instead, monitors with lower resolution show only a window into the map which can be moved with the arrow keys (Figure 18). The resolution giving approximately even aspect ratio is chosen (i.e. showing a circle mostly as round) and no colors are used. All pens draw similarly, including pen 0. Although this screen driver is rather slow in the standard PC computer, its resolution is sufficient to visualize all details of the map on all monitors. BBC SE284 plotter This is a specific driver for the BBC SE284 plotter. The plotter can use several pens that are assembled on its pen rack and referred to by their numbers. Pen number 0 means no pen at all. HPGL compatible plotter The Hewlett Packard Graphics Language (HPGL) is one of the standard vector graphics languages used by many xy-plotters (pen plotters). If your plotter can understand HPGL, choose this driver. Because of its standard nature, the HPGL is suitable also for other purposes. Many word processing programs can read HPGL files and that makes it possible to include DrawMap maps in your text documents directly, without scissors and glue. For that purpose, direct the HPGL data into a disk file (see SETUP section, PLOTTER DRIVERS). Xy-plotters use physical pens and the pen numbers refer to different pens on the pen rack. Pen number 0 means no pen at all. Epson compatible matrix printer Like HPGL, the Epson bit image mode code to make raster images is kind of a standard since many different matrix printers can emulate the Epson printer. The maximum resolution is rather high (240 x 216 dots per square inch - the common laser printers are 300 x 300) and the quality of the drawing is comparable to one produced by a laser printer (see Figures 19 and 20). However, the quality depends a lot on the particular printer used (its pin head and paper feeding mechanisms). Since the matrix printer lacks physical pens, the pen number refers here to the thickness of the line. Pen number one is single dot thickness, two is two dots and so on. With the Epson drive, the pen number 0 does not show. LaserJet II compatible printer As widely as the Epson bit image code is standard within matrix printers, the code of the HP LaserJet II is a standard among laser printers (and some others as well, such as the HP DeskJet). The drawing is a raster image with resolution of 300 x 300 dots per square inch. Also in this drive the pen number refers to line thickness but now so that pen number one means two dots wide line, two is three dots wide and so on. The single dot thickness is too thin for most cases, but you can produce it with pen number 0 (e.g. for miniature maps). Therefore, in order to use no pen at all for parts of the map, you must define Lines=0 in the arc type definitions (see EDIT section). PostScript printer PostScript is a powerful "page description language". Many laser printers use it but it is designed to be used with other equipment as well. Several word processing programs can read PostScript code and include figures made with the PostScript language. PostScript is a very rich language and its vocabulary include vector graphics commands which are the ones DrawMap uses (Figure 20). Since PostScript is a vector language, a laser printer equipped to understand it will produce maps far more quickly than when a raster driver (LaserJet II) is used. The pen numbers refer to line thicknesses exactly as in the LaserJet II Driver. However, since the PostScript unit is not a dot, the line width is defined as a real measure. This means in practice that it is not dependent on the 300 x 300 resolution. The code produced by DrawMap is Encapsulated PostScript, or EPS code. DeskJet printer This driver produces optimized code for the HP DeskJet printer. It is two to three times faster than the LaserJet II driver. Appendix A Editing and creating DNA size standard files (.STD files) The RESTRICTION DATA section calculates the fragments produced from the workfile plasmid when it would be digested with the restriction enzymes indicated. The section can also show a simulated electrophoresis gel where the fragments are shown beside a known series of molecular weight (fragment length) standards. The set of standard fragments varies between different laboratories, but one user has usually a limited set of them. The standard sets are saved on disk as text files and since they are small, they are most easily created from within the DrawMap program (see the RESTRICTION DATA section). The structure of the standard files (the .STD files) is, however, simple and described here if the user wants to edit them with a text editor. The first line contains the name of the standard that appears as a title in the simulated gel. Its maximum length is 20 characters. What follows, starting from the second line, are the fragment lengths in base pairs. They should be in descending order, at least so that the largest is the first one. Be sure not to include extra lines or non-numerical data (except in the first line). They will be ignored but not without complaints. As an example, the set of fragments produced from the phage lambda DNA, digested with the enzymes EcoR1 and Hind3, is shown below. It is included in the DrawMap packet, named L- EH.STD. Lambda EcoR1+Hind3 21227 5143 4975 4271 3522 2023 1906 1584 1374 947 831 564 125 Appendix B Editing and creating restriction enzyme files (.ENZ files) The DNA SEQUENCE section searches restriction enzyme recognition sites from a DNA sequence. The recognition sites for each restriction enzyme can be entered by hand from the keyboard, but that is practical when only a few recognition sites are scanned. The number of known restriction enzymes is quite large and therefore the list of their names and recognition sites is collected into a file. Two such files are provided with the DrawMap program: The file ALL.ENZ contains most commercially available restriction enzymes, with many isoschizomers (recognizing the same sequence) omitted, however. The file 6BASE.ENZ contains a subset of the enzymes in ALL.ENZ, containing those which recognize at least 6-base long sequences. The sources for the enzyme files in this version of DrawMap are: Kessler, C & Manta, V (1990) Gene 92:1-248 and Roberts, RJ (1990) Nucl. Acids Res. 18:2331-2365. The enzyme files are most conveniently updated or edited into subsets with any standard text editor. The characters 1-25 are reserved for the enzymes name and 26-75 for the recognition sequence. For how the alternate bases in the recognition sequence are coded, please refer to Table III in the DNA SEQUENCE section. Keep in mind that the search sequences do not have to correspond to restriction enzymes, they can be anything the user needs. And please do remember: Edit always only copies of the original .ENZ files ! As an example, the file ALL.ENZ is listed below. Aat2 GACGTC Acc1 GTVWAC Acc3 TCCGGA Acy1 GPCGQC Afl2 CTTAAG Afl3 ACPQGT Alu1 AGCT Alw1 GGATC AlwN1 CAGNNNCTG Apa1 GGGCCC ApaL1 GTGCAC Asn1 ATTAAT Asu1 GGNCC Asu2 TTCGAA Ava1 CQCGPG Ava2 GGRCC Ava3 ATGCAT Avr2 CCTAGG Bal1 TGGCCA BamH1 GGATCC Ban1 GGQPCC Ban2 GPGCQC Bbv1 GCAGC Bcl1 TGATCA Bgl1 GCCNNNNNGGC Bgl2 AGATCT Bsa1 GGTCTC BsaA1 QACGTP BsaB1 GATNNNNATC BsaJ1 CCNNGG Bsm1 GAATGC BsmA1 GTCTC BspH1 TCATGA BspM1 ACCTGC Bsr1 ACTGG BssH2 GCGCGC BstE2 GGTNACC BstN1 CCRGG BstX1 CCANNNNNNTGG Cfr10I PCCGGQ Cla1 ATCGAT Dde1 CTNAG Dra1 TTTAAA Dra2 PGGNCCQ Dra3 CACNNNGTG Drd1 GACNNNNNNGTC Dsa1 CCPQGG Eae1 QGGCCP Ear1 CTCTTC Eco47III AGCGCT EcoN1 CCTNNNNNAGG EcoR1 GAATTC EcoR5 GATATC Esp1 GCTNAGC Fnu4H1 GCNGC FnuD2 CGCG Fok1 GGATG Hae2 PGCGCQ Hae3 GGCC Hga1 GACGC HgiA1 GRGCRC Hha1 GCGC Hinc2 GTQPAC Hind3 AAGCTT Hinf1 GANTC Hpa1 GTTAAC Hpa2 CCGG Hph1 GGTGA Kpn1 GGTACC Mae1 CTAG Mae2 ACGT Mae3 GTNAC Mbo2 GAAGA Mlu1 ACGCGT Mnl1 CCTC Mse1 TTAA Mst1 TGCGCA Nae1 GCCGGC Nar1 GGCGCC Nci1 CCSGG Nco1 CCATGG Nde1 CATATG Nhe1 GCTAGC Nla3 CATG Nla4 GGNNCC Not1 GCGGCCGC Nru1 TCGCGA Nsp1 PCATGQ NspB2 GCSGC PflM1 CCANNNNNTGG Ple1 GAGTC PmaC1 CACGTG PpuM1 PGGRCCQ Pst1 CTGCAG Pvu1 CGATCG Pvu2 CAGCTG Rsa1 GTAC Rsr2 CGGRCCG Sac1 GAGCTC Sac2 CCGCGG Sal1 GTCGAC Sau1 CCTNAGG Sau3A GATC Sca1 AGTACT ScrF1 CCNGG SfaN1 GATGC Sfi1 GGCCNNNNNNCCGG Sma1 CCCGGG SnaB1 TACGTA Spe1 ACTAGT Sph1 GCATGC Spl1 CGTACG Ssp1 AATATT Stu1 AGGCCT Sty1 CCRRGG Taq1 TCGA Tth111I GACNNNGTC Xba1 TCTAGA Xca1 GTATAC Xcm1 CCANNNNNNNNNTGG Xho1 CTCGAG Xho2 PGATCQ Xma3 CGGCCG Xmn1 GAANNNNTTC Appendix C Modifying the DMDISP.TXT file Some modifications in the DMDISP.TXT file, the base of the editing screen, may be very valuable for the user. This file, however, is even more in the heart of DrawMap than the standard and enzyme files described in appendixes A and B. Therefore, be extremely careful in not scrambling it and always retain an original copy in a safe place. The file contains some graphical characters and therefore it may not be compatible with all text editors. What you can do with the DMDISP.TXT file is to modify the default data items in new maps. Typically, you may want the comment screen to be, not empty, but have your name and address in it automatically. You may also want to modify the basic map components like character sizes so that they will always appear in the nicer form in new maps. Note that the data in the file DMDISP.TXT never affects the data in existing maps, only in new ones. Not every map component can be predefined. Specifically, the COMPOSITION OF THE PLASMID CIRCLE, the GENES and the SITES cannot be given predetermined values. However, you can predetermine strings or values for the FILENAME, PLASMID NAME and the SIZE. That is more a curiosity, so let's start from the first real thing, the FORM: The FORM determines how the map will be drawn: circular or linear. Internally all maps are circular, so that for example the coordinates 0 and SIZE are the same thing. If you want your maps to be drawn linear by rule, enter "linear" in the FORM box, or anything else than "circular". The LINE TYPES table contains data which you may need to modify. For example, the number of lines in the "heavy" line type may not be sufficient to give a solid line on your plotter and you should increase it. You can also change the name of the LINE TYPE, appearing on the right of the table. This, however, is not really data, carried with each plasmid, but rather a comment on the editing screen. That means that the change made will show while editing old maps, too. The last line of the LINE TYPES table has a back-slash (\) as its first character. This means that the rest of the lines, up to the maximum of twenty, are copies of this line. (When you move in the editing screen of DrawMap, the lines 6-20 exist always in the memory. They are not shown unless their data is different from 0-0-0. The first five lines show always.) If you look at the codes on the right, you will see code 005 on this row. It means that five lines in this table (named E04) was explicitly written before the back-slashed template appears. This may look a bit complicated, but it allows you to extend the list of predefined line types: Insert, between LINE TYPEs 5 and 6, copies of e.g. line 5 and edit their values into what you want, including the comment on the right. Renumber the LINE TYPES and, most importantly, modify the code (originally 005) to correspond to the new number of lines before the back-slashed one. Going forward in the file, the COMPOSITION, GENES and SITES are the tables where modifications of the DMDISP.TXT file have no effect. The suppression list allows them again. Originally it is set to draw everything except the box around the comments. Maybe you want to have the plasmid boxed instead. If you want a particular component to be drawn, write " active " in the box, nicely with lower case letters and two leading and trailing spaces. If you do not want a particular component drawn, write in something else, e.g. "suppressed". In the PICTURE COMPONENTS, you can modify the right column containing the default values. The left column is for the plasmid's own data and not read from the DMDISP.TXT file. The new maps get gets got getting their data directly from the default values of this table. The modifications you make here show also if old maps are edited. They do not affect the old map's data, unless CTRL-D is pressed to reset a particular value for its default. The last box is the COMMENT box where you can write your name or something else you want to appear on all new maps. Note that an eleventh line of the comment box (with the code 010) appears to be available. However, it is not shown on the editing screen. Still, do not remove it from the file since it tells DrawMap that the maximum number of lines (10) was already shown. The last functional line of DMDISP.TXT is the line with the text ----END. Do not remove or modify that. It tells DrawMap where the file ends. What follows, is only comments. In the original file it gives a short description of the structure. What was just described, was the modification of the data which DrawMap has been designed to read from the DMDISP.TXT file for new maps. However, there are more possibilities in tampering with the file. The data tables are formed by the parts of the file where the code at the right has the letter E followed by a number. What is not data in the tables, written inside the boxes, is comment text that you can modify at your will. Between the tables are lines with the code I instead of E. They are intervening lines between the tables and contain only comment text that can be modified. Even more, you can add more intervening lines, or delete away existing ones. For example, if you would prefer different commenting or more elaborate help in the editing screen, you can add it yourself. Finally, you may want to know about the lonely digit code at the right hand side of the texts. That is a color code where 1 stands for green, 2 cyan, 3 blue and 9 a special mix: vertical bars blue, text between them gray, and text after them green. (Do not use code 9 except in tables, however!) Of course, you may have changed the colors green, cyan, blue and gray to something different in the SETUP section. The full listing of DMDISP.TXT follows. Compare it with the listing of the editing screen shown in figure 6. Good luck and don't mess it ! In this section you can establish or edit the coordinates according to 1I01 000 which the circular plasmid map will be drawn. Although limited notes 1 I01 000 are added among the data tables below, reference to the program manual 1 I01 000 is recommended. 1 I01 000 1 I01 000 For information concerning how to move around, press <F1>. 1 I01 000 1 I01 000 To exit, press <ESC>. 1 I01 000 1 I01 000 1 I01 000 1 I01 000 1 I01 000 1 I01 000 1 I01 000 FILENAME 2 I01 000 ┌────────────┐ 3 I01 000 │ │ 9 E01 000 └────────────┘ 3 I02 000 1 I02 000 1 I02 000 PLASMID NAME 2 I02 000 ┌────────────────────┐ 3 I02 000 │ │ 9 E02 000 └────────────────────┘ 3 I03 000 1 I03 000 1 I03 000 SIZE FORM 2 I03 000 ┌──────┐ ┌────────┐ 3 I03 000 │ │ │circular│ 9 E03 000 └──────┘ └────────┘ 3 I04 000 Change with C or L 1 I04 000 1 I04 000 1 I04 000 LINE TYPES OF THE PLASMID CIRCLE 2 I04 000 no thickness lines pen 2 I04 000 ┌──┬─────────┬─────┬────┐ 3 I04 000 │ 1│ 0.000 │ 1 │ 1 │ single 9 E04 000 │ 2│ 0.020 │ 3 │ 1 │ heavy 9 E04 000 │ 3│ 0.030 │ 2 │ 1 │ double 9 E04 000 │ 4│ 0.100 │ 2 │ 1 │ broad double 9 E04 000 │ 5│ 0.000 │ 0 │ 0 │ user defined 9 E04 000 \│ 6│ 0.000 │ 0 │ 0 │ user defined 9 E04 005 └──┴─────────┴─────┴────┘ 3 I05 000 In the table below, reference is made to these line types. 1 I05 000 1 I05 000 1 I05 000 COMPOSITION OF THE PLASMID CIRCLE 2 I05 000 from to type 2 I05 000 ┌───────┬───────┬──┐ 3 I05 000 │ 0 │ 1000 │ 1│ 9 E05 000 │ │ │ │ 9 E05 000 \│ │ │ │ 9 E05 002 └───────┴───────┴──┘ 3 I06 000 To add arrows to the line borders, press > or < for the forward and 1 I06 000 the backward arrow. At contradiction, the arrow at the thicker line 1 I06 000 dominates. CTRL-A removes an arrowhead. 1 I06 000 Overlapping definitions are allowed here and the latest definition 1 I06 000 overrides the others. To compose the overlaps, exit the cursor from 1 I06 000 the table. 1 I06 000 1 I06 000 1 I06 000 1 I06 000 GENES 2 I06 000 from to D name 2 I06 000 ┌───────┬───────┬─┬──────────────────────────────┐ 3 I06 000 │ │ │ │ │ 9 E06 000 \│ │ │ │ │ 9 E06 001 └───────┴───────┴─┴──────────────────────────────┘ 3 I07 000 Enter the genes in a clockwise direction irrespective of 1 007 000 their actual direction. 1 007 000 To add arrowheads to the ends of the genes, press > or < 1 I07 000 while staying in the coordinate box. CTRL-A removes an 1 I07 000 arrowhead. 1 I07 000 The D-box shows the direction of the gene name 1 I07 000 on the map. It is calculated as you exit the line if the 1 I07 000 D-box is empty. You can edit also the D-box. 1 I07 000 1 I07 000 1 I07 000 SITES 2 I07 000 coordinate name type 2 I07 000 ┌──────┬────────────────────┬──────┐ 3 I07 000 │ │ │ │ 9 E07 000 \ │ │ │ │ 9 E07 001 └──────┴────────────────────┴──────┘ 3 I08 000 If the name box is left empty, the previous name is 1 I08 000 copied in the box. 1 I08 000 CTRL-T changes the site type (enzyme, by default). 1 I08 000 1 I08 000 1 I08 000 SUPPRESSION LIST 2 I08 000 status component 2 I08 000 ┌──────────┐ 3 I08 000 │ active │ Draw a box around the map 9 E08 000 │ active │ Write the plasmid name 9 E08 000 │ active │ Write the plasmid size 9 E08 000 │ active │ Write the site coordinates 9 E08 000 │ active │ Write the site names 9 E08 000 │ active │ Draw the site marks 9 E08 000 │ active │ Write the gene names 9 E08 000 │ active │ Draw the gene arcs 9 E08 000 │suppressed│ Draw a box around the comments 9 E08 000 │ active │ Write the comments 9 E08 000 └──────────┘ 3 I09 000 Change status by CTRL-S 1 I09 000 1 I09 000 1 I09 000 PICTURE COMPONENTS 2 I09 000 current default 2 I09 000 value value component 2 I09 000 ┌───────┬───────┐ 3 I09 000 │ │ 0.090 │ sites: character size (y-comp) 9 E09 000 │ │ 1.00 │ character shape (x/y ratio) 9 E09 000 │ │ 0.070 │ genes: character size (y-comp) 9 E09 000 │ │ 1.00 │ character shape (x/y ratio) 9 E09 000 │ │ 0.150 │ name: character size (y-comp) 9 E09 000 │ │ 0.67 │ character shape (x/y ratio) 9 E09 000 │ │ 0.20 │ length of the site mark 9 E09 000 │ │ 1 │ number of blanks after the longest enzyme name 9 E09 000 │ │ 0.80 │ distance of the gene arcs from center 9 E09 000 │ │ 50 │ angle of the gene arrows 9 E09 000 │ │ 80 │ angle of the block arrows on the plasmid 9 E09 000 │ │ 1.00 │ magnification (max ) 9 E09 000 └───────┴───────┘ 3 I10 000 Press CTRL-D to retain the default value. 1 I10 000 1 I10 000 1 I10 000 COMMENTS 2 I10 000 ┌────────────────────────────────────────────────────────────────────────┐3 I10 000 │ │9 E10 000 │ │9 E10 000 │ │9 E10 000 │ │9 E10 000 │ │9 E10 000 │ University of Helsinki │9 E10 000 │ Department of Genetics │9 E10 000 │ Arkadiankatu 7 │9 E10 000 │ SF-OO1OO Helsinki │9 E10 000 │ FINLAND │9 E10 000 │ │9 E10 010 └────────────────────────────────────────────────────────────────────────┘3 I11 000 1 I11 000 1 I11 000 1 I11 000 1 I11 000 1 I11 000 1 I11 000 1 I11 000 1 I11 000 1 I11 000 ----END THE USED PART OF THIS FILE ENDED TWO LINES AGO. THE FILE IS AN IMAGE OF THE DISPLAY FOR EDITING MAP COORDINATES FOR THE DRAWMAP PROGRAM. THE STRUCTURE OF THIS FILE IS: CHARACTER 1 \ MEANS THAT THE LINE IS NOT SHOWN ON SCREEN 1-75 CONTAINS THE TEXT FOR THE SCREEN 76 GIVES THE COLOR OF THE LINE 77 EMPTY 78-80 TELLS WHAT PART OF THE DISPLAY THE LINE BELONGS TO -E MEANS ACTUAL DATA LINE -I MEANS COMMENT LINE 81 EMPTY 82-84 NONZERO AFTER A LINE WHICH CAN BE REPEATED ACCORDING TO A PROGRAM PARAMETER. TELLS THE PROGRAM HOW MANY LINES HAVE ALREADY BEEN USED IN THE BLOCK. Appendix D The structure of the .MAP files The plasmid map files (the .MAP files) need never to be modified by hand when DrawMap is used. Still, they are easily readable text files and their structure is described here. The structure is closely related to the editing screen and is more or less a listing of the contents of the editing boxes and tables. The example map file listed here, PHTT172.MAP, corresponds to the circular map shown in figure 7 and to the editing screen shown in figure 6. The first line is a signature of the file and the DrawMap program reads the version number from this line. The program can always handle .MAP files of older versions, but encountering a file made by a newer version of DrawMap causes an announcement. Reading and comprehending will be tried anyway. The second line contains the plasmid name. Note that the file name is not included in these lines so that renaming the .MAP file with DOS is no problem. The next line contains plasmid size and the tag C or L for circular or linear presentation of the drawing. All the numbers are aligned and right justified. It is necessary to keep them that way. Next follows the data of the LINE TYPES table. It is preceded by the number 20, denoting that the next twenty lines will form the LINE TYPES table. The first column of the table is multiplied here by 1000, compared to the table in the editing screen. After LINE TYPES, the COMPOSITION table is presented, again preceded by the number of lines belonging to this packet, this time seven. The first three columns correspond to what you see in the editing screen: form, to and type. The last one codes the arrow heads, describing the left end arrow (i.e. at the from coordinate ) in the following way: 1: arrow to the left, left type broader 2: arrow to the left, right type broader 3: arrow to the right, left type broader 4: arrow to the right, right type broader Left refers here towards smaller coordinates and right towards larger. Note that the code includes data of which side of the border is broader and which in effect has the arrow protrusion or indentation. The set of lines following describe the GENES, preceded by number of lines. The first two columns correspond to the from and to coordinates, the next two show the presence of arrowheads at these coordinates (0: no, 1: yes), the one character column shows the D or direction-of-name column and what remains is reserved for the name of the gene. Next appear the SITES, lead by the count of lines again. Between the coordinate and the enzyme name is a column which indicates whether the site is an enzyme (e) or a marker (m). In the rest of the file there are no number-of-lines indicators, since the number is fixed in each case. The list of FALSE and TRUE corresponds to the SUPPRESSION LIST (TRUE is active, FALSE is suppressed). The numbers following the suppression list describe the PICTURE COMPONENTS and the last ten lines the COMMENTS. Drawmap version 2.0 map file pHTT172 5923C 20 0 1 1 20 3 1 30 2 1 80 2 2 150 0 1 20 3 3 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 0 7 -2336 0 1 0 0 1180 4 0 1180 1181 5 4 1181 2200 2 0 2200 3587 4 0 3587 5923 1 0 5923 7103 4 0 3 1234 2055 0 1-npt2 3918 4755 0 1-amp 592 592 0 0+P-stem 10 0eEcoR1 12eBamH1 1185eBcl1 1431ePst1 1464ePvu2 2863ePst1 3587eHind3 3678ePvu2 4194eSca1 5743ePvu2 FALSE TRUE TRUE TRUE TRUE TRUE TRUE TRUE FALSE FALSE 0.090 1.00 0.090 1.00 0.150 0.67 0.20 3.00 0.80 50.00 80.00 1.40 The npt2 containing BamH1-Hind3 fragment from tobacco TNT7#3 in pUC8. Teemu Teeri University of Helsinki Department of Genetics Arkadiankatu 7 SF-OO1OO Helsinki FINLAND Appendix E The DrawMap character set The DrawMap character set follows the IBM extended character set for the characters from SPACE (ASCII code 32) forwards. To this, there are three exceptions: characters with codes 246, 249 and 250 are sacrificed for S, R and ■. The listing of the DrawMap character set is (not on this version...) shown at the end of this appendix together with their corresponding IBM set characters and ASCII codes. You can see the three exceptions there. Keyboards do not contain keys for all the special characters. You can access them by pressing and holding down the ALT key and simultaneously typing the characters' code on the numerical key pad. When you release the ALT key, the character appears on screen. Notice that the three DrawMap-specific characters appear in their IBM form on screen - they are special only on drawn maps. The character set is defined by the file DMCHARS. It is a readable text file and simple enough for the user to make modifications in. If you feel that the set is lacking a character you would like to use, you can sacrifice more of the IBM characters for your special purpose. The characters are based on a four by eight grid, shown on the left. The letter A, for example, fits the grid as shown below. If you dig into the DMCHARS file (pick it in a text editor or just type TYPE DMCHARS), you will see rows of three digits interrupted by rows of two digits. The two-digit rows are always headings: they contain first the ASCII code of the character and then the number of lines following belonging to the characters' description. The description, the collection of three-digit lines, is like a collection of imaginary pen strokes. The first two digits define a point on the grid and the last whether the imaginary pen should draw (1) or not (0) when moving there. The definition of the character A, extracted from the file DMCHARS is listed below. You can follow the pen movements on the grid shown above. 65 5 0 0 0 2 6 1 4 0 1 1 3 0 3 3 1 If you want to create a new character for DrawMap, make first a copy of the grid. On the grid, by using straight lines from point to point, design your new character or figure. Next write down a code for the imaginary pen that would draw the new character. You can draw it in any order, but since the maximum number of lines is 30, jumping around should be rationalized at least for complex characters. Count your lines and write the heading: first the ASCII code you want to replace and then the number of lines to follow. The next step is to insert your code in the DMCHARS file. Pick the file in a text editor and search the corresponding ASCII code and character definition. Now replace the lines describing the character by your own. It is important to align your digits as the other digits are aligned in the file. Equally important is to remove all of the old code and write a correct heading line. However, you are not limited to the size of the grid shown above! Characters fitting in the grid will align nicely in written text, all right, but you can use any coordinates between -99 and 127. (In fact the special characters S and R already extend beyond the grid.) For special purposes, it may be useful to know that the consecutive characters in text have two blank grid units between them (i.e., the spacing is 6 grid units). If the maximum of 30 lines for pen code feels limiting, you can compose the complex thing by a character pair, the latter displaced left by 6 grid units ! Finally, a reminder of good working practice: always save the original DMCHARS file in a safe place. It is easy to make disastrous mistakes in editing this file. You wouldn't want to loose your characters, would you ? Appendix F Installation of DrawMap The DrawMap program is supplied on two 360K 5.25 inch floppy disks. In order to run DrawMap, all of the files on these diskettes (except the file INSTALL.BAT) should be copied on one hard disk or larger diskette, in a directory named \DRAWMAP. A hard disk is recommended because of its superior speed. Alternatively, DrawMap can be supplied on a single 1.44M 3.5 inch diskette from which it can be run directly. This diskette, too, contains the installation program for installation on hard disk. The DrawMap diskette 1 contains an automatic installation program. When you run it, give both the source and the destination disk as program parameters. E.g., if you want to install DrawMap on drive C and the DrawMap diskette 1 is in drive A, type INSTALL A: C: Also, if you want to update your DrawMap with a newer version, you can run the installation program. 500 K of space should be free on your disk before you install DrawMap. The program needs the disk also as working space. Some 200K free before starting DrawMap should be safe for most purposes. (It really depends on how huge sequences you analyze with what incredible number of enzymes in the DNA SEQUENCE section). DrawMap is written in Turbo Pascal version 5.0 and it is designed to run in an IBM PC compatible computer. The graphics displays supported are the CGA, EGA, VGA and the Hercules displays. The support of the displays requires the corresponding .BGI file to be found in the \DRAWMAP directory. However, you can dispose of the ones you do not need. DrawMap needs a minimum of 300 K free ram memory to run. Any extra ram, up to 640K, can be used to speed up matrix printer drivers and to analyze an even larger DNA sequence in the DNA SEQUENCE section. If you have extended or expanded memory in excess of the 640K and you could configure it as a virtual disk, DrawMap will run even faster when loaded there. Be careful not to save your map files on the virtual disk since it is volatile and the data is lost when the computer is switched off. DrawMap needs to be started from the directory \DRAWMAP. This does not limit the use of the program in a personal way by different people in the lab. It is very convenient to have personal DOS batch files to start the program and automatically to change the directory. These small files are most easily typed directly from the keyboard, e.g.: copy con DMPETRI.BAT cd \drawmap drawmap \petri\maps CTRL-Z The first line tells DOS to copy from the console (keyboard) a file named DMPETRI.BAT. The next two lines go into the file and the last, CTRL-Z, finishes the copying. Every time DMPETRI is called, the directory will automatically be changed to \DRAWMAP, DrawMap will be started and it will, as the first thing, change the directory to where Petri has his maps saved. Also, if you run DrawMap from a virtual disk, it may be a good idea to start it with a similar type of batch file which will cause automatic saving of the map files on a physical disk. Contact address: Teemu Teeri Institute of Biotechnology University of Helsinki Karvaamokuja 3 SF-00380 Helsinki FINLAND tel. INT-358-0-434 6032 fax. INT-358-0-434 6046 E-mail: teeri@operoni.helsinki.fi teemu.teeri@helsinki.fi