Abstract:
The present invention relates to an automated method of transposon-mediated multiplex sequencing of DNA fragments inserted into a vector. It relates more particularity to an increased efficiency in such automated methods, where the increased efficiency is obtained by screening out before the sequencing those constructs in which the transposon inserted into the vector sequence. This prevents a waste of time and resources in performing reactions sequencing the vector instead of the DNA fragments of interest.

Description:
PRIORITY CLAIM 
     This application is a 35 U.S.C. § 371 filing of PCT Application number PCT/US01/21269 filed on Jul. 5, 2001, which claims the benefit of U.S. Provisional Application number 60/216,381 filed on Jul. 7, 2000. 
    
    
     FIELD OF THE INVENTION 
     The present invention relates to an automated method of transposon-mediated multiplex sequencing of DNA fragments inserted into a vector. It relates more particularly to an increased efficiency in such automated methods, where the increased efficiency is obtained by screening out before the sequencing those constructs in which the transposon inserted into the vector sequence. This prevents a waste of time and resources in performing reactions sequencing the vector instead of the DNA fragments of interest. 
     BACKGROUND OF THE INVENTION 
     The enormous wealth of information that has been acquired from genomic and expressed sequence tag (EST) sequencing in the last 10 years has contributed significantly to efforts to clone full-length cDNA representatives. Although it is anticipated that genomic sequencing projects from human and mouse will be completed in the near future, the transcriptome of these species will remain ambiguous for some time. The complexities involved in predicting, with complete certainty, the splicing program of mRNAs from genomic sequences have compelled additional genomic research focused on obtaining the sequences of full-length cDNAs. In addition, full-length cDNA sequencing efforts are also required for the confirmation of cDNA sequences after methods that involve amplification of the cDNA have been employed for cloning. This scenario is particularly prevalent in genomic centers that are focused on validating gene targets for drug discovery efforts. Clearly, after great expense and effort has been expended, it would be senseless for a putative target to fail the validation process simply because the coding sequence of the target gene was incorrect. Therefore, approaches are required at genomic centers to sequence large numbers of full-length clones quickly, inexpensively, and accurately. For this purpose, Applicants have created a new, integrated high-throughput process called transposon expedited multiplex sequencing (TEMS). 
     In the last 20 years, many methods have been developed for sequencing large inserts to plasmids. However, many of these methods were cumbersome and could not be transferred to high-throughput, automated systems. Sequencing by primer walking is slow, expensive, and often fails since primers are designed to the sequence in a poorly characterized region. Similarly, sequencing by creating a collection of clones by exonuclease digestion from the ends of the target clone is slow, clone specific, and extremely sensitive to the purity and integrity of the template DNA. In addition, the success rate using this approach is quite variable. Shotgun sequencing of clones is a higher-throughput method, however it requires isolating the insert from each clone and then recloning smaller fragments generated by a wide variety of methods. Additionally, shotgun libraries that utilize restriction digests result in a cloning bias and subsequently a non-random distribution of DNA sequence data. 
     Transposon-mediated sequencing can be done by pooling a large number of vectors containing target DNA sequences and randomly inserting a transposon with sequencing primers on each end into the constructs. See Devine, S. E., Boeke, J. E. (1994)  Efficient integration of artificial transposons into plasmid targets in vitro: a useful tool for DIVA mapping, sequencing and genetic analysis , Nucleic Acids Research, pp. 3765-3772; or Kimmel, B., M. J. Palazzola, C. Martin, J. D. Boeke, and S. E. Devine, 1997,  Transposon - mediated DNA sequencing. In Genomic Analysis: A laboratory manual  (ed. E Green, B. Birren, R. Myers, and P. Hieter), Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y., for a description of the method. Traditionally, this method was cumbersome since it required moving plasmids through different host strains for the cloning and transposon-insertion steps. Recently however, several commercial molecular biology vendors have developed in vitro transposition systems to take advantage of the random insertion of a modified transposon (ie. Tn5 etc.). Unfortunately, some of these systems result in a high background of false positives, and are difficult to use with methods to screen positive clones by polymerase chain reaction (“PCR”). Applicants have utilized several of these transposon based sequencing methods and have not experienced any of these difficulties with a modified version of the in vitro GPS-1 transposition system from New England Biolabs. Nevertheless, transposon insertions cannot be directed exclusively to the target DNA of interest and appear in the vector with a high frequency. In an effort to solve this problem and increase the efficiency of transposon facilitated sequencing, Applicants have developed a unique, high-throughput procedure called transposon expedited multiplex sequencing (TEMS). 
     Accordingly, it is an object of this invention to provide a high-throughput, efficient, and inexpensive process for the sequencing of DNA fragments. 
     It is a further object of this invention to provide a high-throughput, efficient and inexpensive process for transposon-mediated sequencing of target DNA fragments which minimizes the amount of non-target DNA sequence generated. 
     It is yet another object of this invention to provide a PCR-based screen to distinguish between the desired constructs with transposons inserted into the target DNA sequence and the undesired constructs with transposons inserted elsewhere. 
     SUMMARY OF THE INVENTION 
     The present invention meets the above objects by providing the following method, which may be automated for further convenience. Multiple DNA target sequences, each cloned into a vector, are pooled and selectable transposons with sequencing primers on each end are inserted randomly into the DNA target-containing vectors. Selected, transposon- and DNA target sequence-containing vectors are then individually screened using a PCR reaction to identify those vectors which have transposons located in the DNA target sequence. The PCR reaction uses primers located at each end of the vector sequence and is optimized to provide sufficient extension time for the PCR polymerase to efficiently produce a product the length of the vector, but insufficient extension time for the PCR polymerase to efficiently produce a product the length of the vector plus the transposon. Therefore, significant amounts of PCR product will only be produced for vectors containing the transposon in the DNA target sequence and not the vector. The presence or absence of a significant amount of PCR product for each PCR reaction can be quickly determined by the use of a quantitative fluorescent dye selective for double stranded DNA (“dsDNA”). Vectors identified by a significant PCR product in the prescreen are then individually sequenced using the sequencing primers on each end of the transposon to read out into each DNA target sequence. The raw DNA target sequences of individual sequencing reactions can be combined to determine the full sequence of each of the DNA targets in the pool. 
     The parallel processing of clones greatly increases the speed in which reactions can be set up and sequenced. Additionally, the process does not rely on any particular vector and does not require any recloning steps. Most important for overall efficiency, sequencing of the vector backbone is minimized or eliminated with the screening step. Automation of each of the steps of the instant process can be readily achieved using equipment available to those in the art of automated DNA sequencing. 
    
    
     
       BRIEF DESCRIPTION OF THE DRAWINGS 
         FIG. 1  is a diagram of the steps of TEMS. 
         FIG. 2  shows the sequence of GPS-Apra transposon vector (SEQ ID NO: 1). 
         FIG. 3  shows the sequence of GPS-Apra-2 μm-URA3 transposon vector SEQ ID NO: 2). 
         FIG. 4  is a picture of an electrophoresis gel stained to show the products of PCR reactions using various polymerases to multiply the vector portions of the transposon- and target- DNA-containing vectors. 
         FIG. 5  is a picture of an electrophoresis gel stained to show the products of PCR reactions having too great an extension time to eliminate an approximately 9 kb product. 
         FIG. 6  is a picture of an electrophoresis gel stained to show the products of PCR reactions at a variety of extension temperatures and having different numbers of cycles. 
         FIG. 7  is a picture of an electrophoresis gel stained to show the products of PCR reactions and a table of the PICOGREEN® results for the same PCR reactions. 
     
    
    
     DEFINITIONS 
     As Used Herein: 
     A “vector” is any DNA construct which replicates in a cell and has an insertion site at which unknown DNA sequences can be inserted. 
     “Selectable”, in reference to a vector or transposon, means that the vector or transposon carries a phenotype that can be used to identify cells transformed with the vector or transposon. Preferably, the phenotype allows the transformed cells to survive in conditions in which non-transformed cells cannot. 
     A “target DNA” or “target DNA sequence” is a DNA molecule of known or unknown sequence which the operator of the method desires to sequence. 
     A “representative number of individual transformants” is a minimum number of individual transformants which ensures that for each target DNA in the pool there will be a sufficient number of transformants containing insertions of the transposon into that target DNA to provide a desired number of independent sequencing determinations of each base in that target DNA. 
     “Substantial amounts of dsDNA” in regard to PCR products is an amount of dsDNA that exceeds a predetermined threshold. The predetermined threshold can be identified by evaluating the variability of PCR products found within PCR reactions with several constructs which are known to contain the transposon inside or outside the vector sequence. 
     DETAILED DESCRIPTION OF THE PREFERRED EMBODIMENTS 
     The present invention provides a method that can be efficiently automated for sequencing multiple target DNAs in parallel. In the method, each target DNA sequence is inserted into a selectable vector, preferably a plasmid, at identical insertion points in the vector sequence. It is important that all target DNAs are inserted into the same vector or, if different vectors are used, that each vector is substantially the same size and has identical sequences around the insertion point so that one set of primers can be used to amplify all the vectors by PCR reaction. 
     The vectors containing each of the multiple target DNA sequences are pooled in ratios based on the length of each target DNA sequence, so the pool contains substantially equal amounts of each kb of each target DNA sequence. The ratios for each vector to be included in the pool can be determined by determining the lengths of each target DNA sequence (for instance, by electrophoresis against standards size markers on an agarose gel), and adding to the pool a set amount of each vector for every kb in length of the target DNA sequence in that vector. 
     A transposon-insertion reaction is then performed on the pool to randomly insert a selectable transposon into the target-DNA containing vectors. Although this step could be performed by traditional, in vivo, transposon insertion, that would require moving a plasmid through more than one cell type. In vitro transposon-insertion reactions are much simpler and faster. The transposon must carry a selectable marker and must be of sufficient size to enable PCR conditions to be established that efficiently multiply a dsDNA fragment the size of the vector, but do not significantly multiply a dsDNA fragment the size of the vector plus the transposon. Preferably, the transposon is about equal to or greater than the vector in length. Most preferably, the transposon is equal to or greater than 5/4 the length of the vector. Particularly preferably, the transposon is equal to or greater than 5/3 the length of the vector. Where the vector is a bacterial plasmid, the transposon is preferably at least about 3 kb, most preferably at least about 4 kb and particularly preferably greater than or equal to about 5 kb. 
     The pool of vectors from the transposon-insertion reaction is then used to transform cells and the transformants are grown under conditions which select for the transposon. Selected transformants are isolated and grown into cultures. The number of isolated transformants grown into cultures depends on the number and size of target DNA sequences in the pool. Enough transformants must be isolated and grown to ensure that for each target DNA sequence, the isolated transformants will include enough individual insertions of the transposon into that particular target DNA sequence to provide several fold independent sequence determinations of each and every base in that target DNA sequence. To ensure against errors, those of skill in the art often seek to obtain a 6-fold coverage of sequence data, although they may opt for more or less, as the situation merits. When attempting to obtain 6-fold coverage, as a general rule of thumb, 18 clones will need to be actually sequenced per 1 kb of nucleotides to obtain this coverage. However to actually sequence 18 clones, a greater number of transformants will have to isolated and grown, because the transposon will not have integrated into the target DNA in every case, but will have randomly inserted over the whole target DNA-containing vector. Therefore, the number 18 is multiplied by the likelihood that the transposon inserted into the target DNA sequence. So, to obtain 6-fold sequencing coverage, for each target DNA sequence in the pool, a number of transformants to be isolated is equal to: the length of the target DNA sequence in kb times 18, times the ratio (size of vector)/(size of DNA target sequence). 
     Each culture from a selected transformant then has a PCR reaction performed on its DNA. The PCR reaction uses primers complementary to the 3′ ends of the vector sequence at the insertion point, which allow PCR multiplication of a fragment the size of the entire vector sequence. The reaction conditions of the PCR reaction are optimized to efficiently produce a fragment the length of the vector, but not to efficiently produce a fragment the length of the vector plus the transposon. The optimization of PCR conditions for any particular vector and transposon combination according to this invention can be determined by one of skill in the art through routine experimentation, as guided by such reference works as Kimmel, B., M. J. Palazzola, C. Martin, J. D. Boeke, and S. E. Devine, 1997,  Optimizing PCR Assays, Methods for Improving PCR, Detecting and Characterizing PCR products, Protocols for Detecting and Characterizing PCR Products. In Genomic Analysis: A laboratory manual  (ed. E Green, B. Birren, R. Myers, and P. Hieter), Cold Spring Harbor Laboratory Press, Cold Spring Harbor, N.Y.; and Cha, R. S. and Thilly, W. G. (1995) in:  PCR Primer , Dieffenbach, C. W. and Dveksler, G. S. (eds.), CSH Press, New York. The particular DNA polymerase used for PCR should not be limiting for the method, although the choice of polymerase may help to optimize the reaction. Generally, the elongation temperature and/or time of the PCR are varied to achieve the desired exclusion of the vector plus transposon sized product. For a demonstration of optimization, see Example 2. 
     The amount of product produced in each PCR reaction is then measured, preferably optically. Optical measurement could be made by any method which distinguishes dsDNA from nucleotides, but is preferably made using a fluorescent dye specific for dsDNA. dsDNA specific dyes include the bis-benzimide dye Hoechst 33528 and the cyanine dyes of Molecular Probes, Inc, Eugene, Oreg., including PICOGREEN®. PICOGREEN® is preferred, due to its sensitivity and selectivity for dsDNA. The measured value of fluorescence is compared to a predetermined threshold level for determining whether a significant amount of dsDNA PCR product is present. The threshold level of fluorescence is set experimentally using positive and negative control PCR templates of the size of the vector alone and the vector plus the transposon, under the same PCR conditions that will be used to screen the isolated transformants. 
     Those transformants corresponding to PCR reactions which did not produce substantial amounts of dsDNA are not sequenced, because they contain the transposon in the vector sequence. Transformants corresponding to PCR reactions which produce substantial amounts of dsDNA contain the transposon in the target DNA sequence and are sequenced. Two sequencing reactions are performed for each transformant, using primers from each end of the transposon to read the sequence of the target DNA sequence surrounding the transposon. The sequencing reactions can be performed by any of the known methods of the art. 
     Once sequence data has been collected from all the transformants which passed the PCR screen, the sequences must be assembled into all the individual members of the pool of target DNA sequences. This can be accomplished by methods of computer sequence analysis known in the art, and the exact manner is not limiting on this invention. 
     The advantages of the instant method include speed, efficiency and an ability to automate the process. Particularly, the instant method provides a quick PCR screen that allows for elimination of those unproductive transformants which have the transposon inserted into the vector sequence and would yield mainly vector sequences if sequenced. The PCR screen is fast, can be automated and does not require any isolation of the PCR product, such as running an agarose gel to determine its size. The use of a pool of target DNAs allows a single transposon reaction and a single transformation to be performed, instead of requiring one for each target DNA sequence. 
     EXAMPLES 
     Example 1 
     Choosing a Transposon to Fit a High-Throughput Screening Process 
     Original Transposon from New England Biolabs 
     The Genome Priming System Kit from New England Biolabs, 32 Tozer Road, Beverly, Mass. 01915 (“NEB”) was used to initially prove that a transposon inserted randomly into DNA targets could be an efficient way to completely sequence the targets with a great degree of accuracy. Supplied with the kit was one of two transposons that contained the kanamycin resistance gene. However, kanamycin is a fairly common resistance marker, and if a target DNA sequence was already cloned into a kanamycin-selectable vector, then either a different transposon or recloning of the target DNA sequence would be required. The kit provided another transposon that contained the chloramphenicol resistance marker, but that, too, is fairly common. Therefore, the transposon should be modified to contain an uncommon resistance marker, such as apramycin, to avoid additional cloning steps and reduce human error in choosing the correct transposon for each DNA target. The GPS-Apra transposon ( FIG. 2 ) was constructed by modifying the NEB pGPS1 transposon. 
     Screening Method Using the Modified Transposon, GPS-Apra 
     Initial experiments showed that a screening process could identify from transformants selected for the transposon those transformants containing the transposon in the target DNA sequence and not the vector. This reduces costs by eliminating unproductive sequencing of the vector sequence. The original NEB pGPS1 transposon was 2.614 kb with ˜1.7 kb of that, with priming sites at each end, being randomly inserted into the target DNA. By PCR amplification of the 3.0 kb vector using complement M13F and complement M13R primers, two distinct PCR products could be visualized on a slab gel. A 3.0 kb PCR product indicates that the transposon must be in the target DNA sequence, since the vector is 3.0 kb. A 4.7 kb PCR product indicates a vector (3.0 kb) containing the transposon (1.7 kb). Therefore, clones containing the transposon in the target DNA sequence could be identified by the presence of 3.0 kb PCR products on the gel. 
     To demonstrate identification of clones containing the transposon in the insert, colonies were selected from the transformation following the transposon reaction and inoculated into media containing both antibiotics for selection, apramycin and the plasmid antibiotic. The culture was grown up overnight and PCR was done the following day by kerplunking approximately 1 ul of culture into a PCR cocktail in a 96 well plate. The PCR cocktail included the Amplitaq enzyme and reagents from PE Corporation, PE Corporation, 761 Main Avenue, Norwalk, Conn. 06859. The conditions for PCR were standard {95 C for 5 min, (95 C for 30 sec, 54 C for 1 min, 72 C for 6 min, 30 cycles), 72 C 1 min, 4 C forever}. After completion of the cycle (approximately 2.5 hr), gel electrophoresis was done using 8 ul of the 50 ul PCR reaction on a standard size gel. There was a clearly detectable size distinction between the PCR products from vector sequence without the transposon and vector sequence including the transposon. 
     To maintain a high-throughput for the sequencing reactions, however, electrophoresis would have to occur on large gels that could hold hundreds of samples at one time. On these large gels, the difference between a 3 kb and a 4.7 kb fragment would be difficult to reproducibly detect with an automated system. Also, gel electrophoresis was very time consuming and would interfere with performing the screen in a high-throughput manner. 
     In a search for other, high-throughput methods, fluorescent detection of dsDNA was settled on as reproducible and less time consuming. The PICOGREEN® assay seemed particularly convenient. However, fluorescent detection of dsDNA cannot distinguish between different size fragments, so the PCR reaction had to be altered so that the presence or absence of any PCR product indicates the position of the transposon in the target DNA containing vector. If only clones with the transposon in the target DNA sequence produced a dsDNA PCR product, then the PICOGREEN® dsDNA dye would fluoresce at a high level for only the desired clones. The wells that contain the transposon in the vector would not amplify a significant dsDNA product and would result in a low level of fluorescence. A cutoff level of fluorescence between desired and undesired clones can be determined by the use of known samples. 
     A variety of PCR conditions were tested by lowering the elongation temperature, but the 4.7 kb band would not consistently drop out, without having an increase of false positives. It was decided that if the transposon could be modified again to greatly increase its size, then PCR conditions could be developed that would consistently drop out the upper, transposon-containing band, thereby lowering the false positive rate. A large “stuffer” gene that would not effect the transposon reaction in a negative way was sought. A yeast 2 um plasmid with the URA3 gene met the size criteria and could also be used in yeast experiments in the future. Therefore, a GPS-Apra-2 um-URA3 transposon plasmid ( FIG. 3 ) was constructed having a total size of 6.1 kb, including the transposon of ˜5.0 kb. The PCR conditions were altered successfully to drop out the clones with the transposon in the vector and the transposition reaction was not affected. See Example 2. 
     Example 2 
     Optimization of PCR Conditions to Reduce False Negative and False Positive Results 
     Basic PCR Concept 
     This screen is based on PCR cycling conditions that have been specifically optimized to amplify a 3.9 kbp fragment of the entire vector DNA. In this case, the vector was PCR4Blunt-TOPO from Invitrogen, 1600 Faraday Ave, Carlsbad, Calif. 92008. If the vector has the 5 kbp transposon inserted into it, its size will be increased to 8.9 kbp, which is too large to be amplified under the optimized PCR conditions. 
     The primer sequences selected to amplify the vector portion of the Jones are the complement sequences of the universal primers M13F(−20) and M13R. The sequences are as follows 5′-ACTGGCCGTCGTTTTAC-3′ SEQ ID NO: 3) and 5′-CATGGTCATAGCTGTT-3′ (SEQ ID NO: 4). This amplification is illustrated in  FIG. 1 . 
     Background on the Development of the 384-Well Format 
     In order to screen transposon reactions from pools containing multiple clones it was necessary to develop a screen that was both quick and cost efficient. Initial development attempts were based on the 96-well protocol. To change to a 384-well plate, all reagent volumes were halved to accommodate the smaller well volume. However, these conditions proved to be less than ideal due to the high number of PCR failures that were being observed. A search for PCR reagents and conditions that were more robust for this format was undertaken. The results of experiments that tested a wide range of enzymes and thermocycling conditions will be described in the following sections. 
     384-Well PCR Optimization Process 
     Polymerase Selection 
     A quick screening of a variety of PCR kits from several vendors was done to determine a 384-well replacement for the PE Corporation AmpliTaq polymerase that had been used in the 96-well format. The following pcr kits were tested: Clontech&#39;s Advantage cDNA PCR kit, Epicentre&#39;s Failsafe PCR system, and three kits from Takara; LA Taq, Ex Taq, and Z Taq. (Clontech Laboratories Inc. is located at 1020 East Meadow Circle Palo Alto, Calif. 94303-4230; Epicentre Technologies is located at 1402 Emil Street, Madison, Wis. 53713 ; and Takara Shuzo Co., LTD has a business address of Biomedical Group Seta 3-4-1, Otsu, Shiga, 520-2193, Japan.) Samples tested represented 30 pooled DNA targets. They were cloned into pBluescript SK—(3.0 kb) from Stratagene, 11011 North Torrey Pines Road, La Jolla, Calif. 92037. The growth time was 20 hr in 384 well format. Based on preliminary data the Z-taq system was chosen as the enzyme to pursue due to properties it possessed which made it ideal for use in a high-throughput system like TEMS. See  FIG. 4 , which shows a stained electrophoresis gel on which the PCR products of the samples have been run. 
     Reagent Optimization 
     It was also desirable to decrease the cost per reaction of the PCR screen. Table 2, shown below, summarizes the various experiments that were done to test the amount by which each of the various reagents could be lowered without compromising the results. 
                                   TABLE 2                   Table summarizing the various PCR cocktail       ingredients that were tested during the optimization process.            Variable Tested   Condition Tested   Optimal Result               Z- Z-Taq polymerase   0.625, 0.313, 0.156 Units   0.313 Units       10X Z-Taq Buffer   1x, 0.5x   1x       Primers   2.5, 5, 10 pmol   5 pmol       Primers   cM13f &amp; cM13r   cM13f &amp; cM13r           cT3 &amp; cT7           dNTP&#39;s   100, 150, 200 μM   150 μM                    
Based on the above experiments the following optimized reaction cocktail mix (per sample) was determined:
     ddH 2 0: 17.875 μL   10× Z-Taq buffer: 2.5 μL   dNTP mixture: 1.5 μL   template DNA: 1 μL (deposited using a Kerplunker #96/384, manufactured by Nalge Nunc International, 75 Panorama Creek Drive, Rochester, N.Y. 14625, and Pin Replicator #250520/250393)   Z-Taq DNA polymerase: 0.125 μL (0.3125 Units)   cM13f (5 pmol/μL): 1 μL   cM13r (5 pmol/μL): 1 μL   
     Optimization of Thermocycler Conditions 
     Initial thermocycling conditions used were based on recommendations found in the Takara literature. These conditions were: 
     
       
         
               
               
               
             
               
               
             
           
               
                   
                   
               
             
             
               
                   
                 1. denature: 
                 98° C. for 5 seconds 
               
               
                   
                 2. anneal: 
                 55° C. for 10 seconds 
               
               
                   
                 3. extension: 
                 72° C. for 60 seconds (15.4 seconds/kb) 
               
             
          
           
               
                   
                 4. go to 1, 30 times 
               
               
                   
                 5. 4° C. until the PCR reaction is evaluated. 
               
               
                   
                   
               
             
          
         
       
     
     The results of using these conditions are shown in  FIG. 2 . From that data, it was decided that the annealing temperature should be lowered so as to try and decrease the reaction specificity and thus increase the number of positives that are amplified. In the next experiment the annealing temperature was lowered to 52° C. Although this helped with the overall reaction results, it was discovered that using an extension time of 15.4 seconds per kbp resulted in the amplification of vector containing the transposon insertion. See  FIG. 5 , which shows a stained electrophoresis gel on which PCR products from 47 transformants selected after transposon insertion in target DNA-containing pBluescript SK- and grown for 20 hours in wells of a 384 well plate were run. The appearance of a 9 kbp band, believed to be the amplified product of vector containing the transposon, is the result of an excessive extension time. 
     Additionally, an annealing temperature gradient between 48° C. and 68° C. was tested to confirm that 52° C. was indeed the optimal temperature to use for this PCR. In the same experiment the number of cycles was also tested. 30, 35, 40, and 45 cycles were tested. From the results of that experiment it was determined that the number of cycles need to remain low to avoid background noise. From the 48° C. and 68° C. gradient the 52° C. annealing temperature was reconfirmed as being optimal. The temperature is not too low that it becomes non-specific and not too high that it risks approaching the 56° C. temperature at which the PCR begins to fail. These results are shown in  FIG. 6 , a picture of a stained electrophoresis gel, where each depicted product represents amplification of the control pBluescript SK- vector at 2.5 ng per well, in a 384 well format with 25 ul PCR cocktail volume. Based on the above data, the thermocycling conditions were determined to perform optimally using the following cycle. 
     
       
         
               
               
               
             
               
               
             
           
               
                   
                   
               
             
             
               
                   
                 1. denature: 
                 98° C. for 5 seconds 
               
               
                   
                 2. anneal: 
                 52° C. for 10 seconds 
               
               
                   
                 3. extension: 
                 72° C. for 30 seconds (7.7 seconds/kb) 
               
             
          
           
               
                   
                 4. go to 1, 35 times 
               
               
                   
                 5. 4° C. until evaluation of the PCR reaction. 
               
               
                   
                   
               
             
          
         
       
     
     Since evaporation was found to be a problem in the 384-well plates, rubber ‘P’ seals from MJ Research, 590 Lincoln Street, Waltham, Mass. 02451, are placed over sealed plates before thermocycling begins. Along with this, and as recommended by the manufacturer, the lid temperature is set to 85° C. 
     Table 3, shown below, provides a summary of the various PCR thermocycling conditions tested during the optimization process. 
                                       TABLE 3                   Summary of the PCR thermocycling       conditions that were tested during the optimization.                Variable Tested   Condition Tested   Optimal Result                       Annealing   38° C.–68° C.   52° C.           Temperature               PCR cycle   30, 35, 40, 45   35                        
Screening for Positive Clones Using the dsDNA Quantitation Reagent PICOGREEN®
 
     To bypass the labor-intensive task of gel electrophoresis, the TEMS PCR screen utilizes the dsDNA quantitation reagent, PICOGREEN®. The PICOGREEN® is diluted to a working dilution of 1:150 in 1× TE buffer. This dilution was found to be optimal, although it is slightly more concentrated than the 1:200 dilution recommended in the manufacturer&#39;s protocol. 
     25 μL per well of 1:150 PICOGREEN® is aliquoted into black 384-well plates using a Robbins Hydra 96 Dispenser from Robbins Scientific, 1250 Elko Drive, Sunnyvale, Calif. 94089-2213. 5 μL per well of each PCR reaction is then added to the PICOGREEN®, again using the Hydra Dispenser. The plate is then immediately placed into a Molecular Dynamics Gemini Fluorescence Plate Reader and the plate is then mixed for 10 seconds before its fluorescence signal is measured. 
     For the assay to function as a screen, there must be a clear difference in the fluorescence signal between positive and negative wells. PCR product amounts of 1.3, 2.5, 5, and 10 μL were tested to determine the greatest assay range of positive signal to background. Results showing that 5 μL of PCR product into 25 μL of PICOGREEN® is the optimal condition to use is shown in Table 4. 
     
       
         
               
             
               
               
               
               
               
               
               
               
               
               
               
               
               
               
               
             
               
               
               
               
               
               
               
               
               
               
               
               
               
               
               
             
               
               
               
               
               
               
               
               
               
               
               
               
               
             
               
               
               
               
               
               
               
               
               
               
               
               
               
             
           
               
                 TABLE 4 
               
               
                   
               
               
                 Fluorescence signal detected using the PICOGREEN ® assay with various amounts of 
               
               
                 PCR product. The 24 PCR products are from samples representing a pool of 11 DNA targets 
               
               
                 with a sizes up to 4.5 kb cloned into the vector PCR4Blunt-TOPO. The transposon used was 
               
               
                 pGPS-Apra-2 uM-URA3. 
               
               
                   
               
             
             
               
                   
               
             
          
           
               
                 uL 
                   
                   
                   
                   
                   
                   
                   
                   
                   
                   
                   
                   
                   
                   
               
               
                 PCR 
                 1 
                 2 
                 3 
                 4 
                 5 
                 6 
                 7 
                 8 
                 9 
                 10 
                 11 
                 12 
                 13 
                 14 
               
               
                   
               
             
          
           
               
                 1.3 
                 353 
                 287 
                 206 
                 987 
                 180 
                 345 
                 1734 
                 351 
                 171 
                 312 
                 309 
                 237 
                 1102 
                 308 
               
               
                 2.5 
                 839 
                 827 
                 495 
                 1924 
                 412 
                 751 
                 2941 
                 694 
                 397 
                 710 
                 711 
                 413 
                 2129 
                 541 
               
               
                 5 
                 1489 
                 1503 
                 835 
                 2769 
                 635 
                 1450 
                 3703 
                 1640 
                 813 
                 1220 
                 1447 
                 882 
                 2991 
                 1198 
               
               
                 10 
                 1806 
                 2234 
                 1775 
                 3023 
                 1354 
                 2099 
                 3870 
                 2112 
                 1378 
                 2095 
                 1909 
                 1746 
                 3401 
                 1882 
               
               
                   
               
             
          
           
               
                   
                 uL 
                   
                   
                   
                   
                   
                   
                   
                   
                   
                   
                 high- 
               
               
                   
                 PCR 
                 15 
                 16 
                 17 
                 18 
                 19 
                 20 
                 21 
                 22 
                 23 
                 24 
                 low 
               
               
                   
                   
               
             
          
           
               
                   
                 1.3 
                 202 
                 245 
                 843 
                 134 
                 126 
                 318 
                 223 
                 308 
                 635 
                 223 
                 1608 
               
               
                   
                 2.5 
                 456 
                 549 
                 1713 
                 313 
                 217 
                 634 
                 407 
                 690 
                 1434 
                 552 
                 2724 
               
               
                   
                 5 
                 934 
                 1003 
                 2560 
                 624 
                 552 
                 1259 
                 1112 
                 873 
                 2341 
                 1116 
                 3151 
               
               
                   
                 10 
                 1681 
                 1574 
                 2902 
                 1197 
                 983 
                 1637 
                 1642 
                 1560 
                 2967 
                 1333 
                 2887 
               
               
                   
                   
               
             
          
         
       
     
     The signal output generated by the fluorescence reader is then exported to a histogram display, and a cutoff value for positive clones is assigned from the histogram. Using the current conditions, the cutoff generally falls between 1000-1500. 
     A Genesis RSP 150 TECAN robotics station (TECAN U.S. INC., P.O. Box 13953, Research Triangle Park, N.C. 27709) was used to generate 96-deep-well plates containing cells from the clones identified by the screen as having the transposon in the target DNA sequence. Cells from each positive clone are placed in Superbroth and the appropriate antibiotics (dual selection) in one of the wells. These plates are grown and then the cultures are submitted for automated sequencing. 
     Example of the Optimized PCR Screen Technique for 384-Well Plates 
     Use Q-Bot to pick colonies of the transposon containing clones into Genetix 384-well shallow-well plates containing 65 μL per well of Superbroth plus appropriate antibiotic. Place plates into a humidified 37° C. incubator for 19-22 hours. Aliquot 25 μL per well of sterile 50% glycerol into the growth plates using a Multidrop 384 115V liquid dispenser (Labsystems Inc., 8 East Forge Parkway, Franklin Mass. 02038). Using the glycerol plate as the template, set-up PCR using the following recipe:
         ddH 2 0: 17.875 μL   10× Z-Taq buffer: 2.5 μL   dNTP mixture: 1.5 μL   template DNA*: 1 μL (using the Kerplunker, pin-tool)   Z-Taq DNA polymerase: 0.125 μL (0.3125 Units)   cM13f (5 pmol/μL): 1 μL   cM13r (5 pmol/μL): 1 μL   *To ensure that the Kerplunker is sterile it should be stored in 70% ethanol and flamed before use.
 
Placed the PCR reaction plate into a thermocycler and start the following cycle:
       

     
       
         
               
               
               
             
               
               
             
           
               
                   
                   
               
             
             
               
                   
                 1. denature: 
                 98° C. for 5 seconds 
               
               
                   
                 2. anneal: 
                 52° C. for 10 seconds 
               
               
                   
                 3. extension: 
                 72° C. for 30 seconds (7.7 seconds/kb) 
               
             
          
           
               
                   
                 4. go to 1, 35 times 
               
               
                   
                 5. 4° C. until the PCR reaction is evaluated. 
               
               
                   
                 Total cycling time: 1 hour, 18 minutes, 30 seconds. 
               
               
                   
                   
               
             
          
         
       
     
     While the reaction is underway, thaw the PICOGREEN® reagent at room temperature. 
     Prepare a 1:150 dilution of PICOGREEN® in 1× TE Buffer. Prepare 10 mL per 384-well plate. Use the Robbins Hydra to aliquot 25 μL per well to an entire 384-well black plate. Use the Robbins Hydra to dispense 5 μL per well of the PCR reaction into the PICOGREEN® plate. Immediately place the plate into the fluorescence plate reader and mix by shaking for 10 seconds. Export the fluorescence signal data to a floppy disk. Import data into an Excel macro and generate a rearray list of positive clones using 1500 as the threshold. See  FIG. 7  for an example of final PICOGREEN® data obtained from a PCR screen. Open the rearray list in the TECAN robot and rearray clones from the glycerol stock plate into a 96-well deep-well plate containing Superbroth and appropriate antibiotics. After the plates have been incubated, the cultures in them are sequenced in an automated process. 
     Example 3 
     Transposon Expedited Multiplex Sequencing of Unknown Sequences in Vector PCR4Blunt-TOPO 
     Transposon Reaction 
     The transposon reaction was performed using the Genome Priming System (GPS) kit from New England BioLabs. All of the components provided in the kit were used with the exception of the transposon GPS1. The transposon utilized was a modified version of GPS1. Two variations were generated. In one variant, pGPS-Apra, the existing resistance marker has been replaced by the apramycin resistant gene. This was performed to ensure that the vector could be used to sequence any vector regardless of resistance marker. In another variant, pGPS-Apra-Y2 um a “stuffer” region containing the yeast 2 um replication origin was cloned into the transposon thus increasing its size to 5 kb ( FIG. 6 ). This alteration was created in order to improve the efficiency of the process by screening out transpositions into the vector backbone. The reaction was transformed by electroporation into DH10B  E. coli  competent cells and plated on Luria-Bertani (1.0% bacto-tryptone, 0.5% bacto-yeast extract, 1.0% NaCl, pH 7.0) agar plates containing the appropriate antibiotics (aprarnycin (100 μg/ml)/kanamycin (50 μg/ml)) for selection of clones harboring the transposon. The growth period is 20-22 hours. 
     TEMS (Transposon Expedited Multiplex Sequencing) 
     The size of all target DNA sequences subjected to TEMS was evaluated by restriction digest of the target DNA-containing vectors with NotI. Plasmid sets containing target DNA sequences of various sizes contained in the same vector backbone were pooled. Equimolar concentrations were calculated for each target DNA sequence prior to pooling. The transposon reaction was performed treating the pooled DNA template as a single template. For six-fold coverage of each base of each target DNA sequence, the total size of each target DNA sequence was multiplied by our standard factor of 18 clones per 1 kb of sequence to determine the number of randomly selected clones to sequence. Based on the total size of the vector and the total size of the target DNA sequence, a probability of the location of the transposon insertion was calculated. Multiplying this factor with the number of clones for six-fold coverage determines how many clones to randomly select and subject to the PCR screen. 
     The calculated number of colonies were selected and inoculated into Superbroth (bacto-tryptone, yeast extract, NaCl, NaOH) media containing the appropriate antibiotics on 96 or 384 well culture plates. These culture plates were grown overnight without shaking for 18-22 hours depending on the format of the growth plate (96/384 well). Glycerol stocks were made for temporary storage of the plate. 50% glycerol was added directly to the plate and mixed. This allowed indefinite storage in −80 C. 
     Screening out Vector Insertions by PCR 
     The primer sequence selected to amplify the vector portion of the clones for screening were the complement sequences of the universal primers M13F(−20) and M13R The sequence is as follows: 5′-ACTGGCCGTCGTTTTAC-3′ (SEQ ID NO: 3) and 5′-CATGGTCATAGCTGTT-3′ (SEQ ID NO: 4). Culture PCR was assembled with the following conditions: the template was deposited into the PCR reaction reagent preparation using a pin replicator tool which aliquoted approximately 1 μL. For the 96-well format, the 10 times PCR buffer composition was 100 mM Tris-HCl pH 8.3; 500 mM KCl: 15 mM MgC12; 0.01% w/v gelatin. Five picomoles of the forward primer and five pmoles of the reverse primer were used in each reaction. The dNTP concentration in the reaction was 2.5 mM final concentration. The quantity of Taq polymerase added to each reaction was 0.1 units. All reactions were carried out in a total volume of 50 μl. The 384-well format PCR was done in a total volume of 25 μl using the TaKaRa Z-Taq kit obtained from Panvera Corporation, 545 Science Drive, Madison, Wis. 53711. This kit consists of Z-taq polymerase (2.5 units/μL), 10× Z-Taq buffer containing a 30 mM concentration of Mg2+, and a JNTP mixture (2.5 mM each). Thermocyclers were run with a heated lid (MJ Research). This PCR cycle was designed to amplify only the vector without the transposon due to the short elongation time. Black PCR plates were used so that the fluorescent analysis could later be performed directly in the plates. 
     Analysis Conditions Using PICOGREEN® 
     Upon completion of the PCR, 25 ul of PICOGREEN® was added the PCR plate. A dilution of PICOGREEN® stock 1:200 in 1× TE (tris-acetate, EDTA) buffer at 50 ul volume was mixed with 10 ul of PCR reaction. The plate was read in a spectrofluorometer where the molecules are excited at 480 nm and the signal is emitted at 540 nm. The PCR products fluorescing above a predetermined threshold were the positive clones to be sequenced. The threshold was experimentally determined using known constructs containing the transposon either in the vector or in an insert to the vector. The positive clones were sorted and compressed into a format suitable for array by the TECAN robotic arm. Glycerol stocks were inoculated into the 96 deep well plate containing 1.5 ml of Superbroth (bacto-tryptone, yeast extract, NaCl, 5N NaOH) and appropriate antibiotics. These cultures were grown for a 24 hour time period and then the DNA targets from the cultures are sequenced using the primers at either end of the transposon. 
     Sequence Assembly 
     After vector trimming and base calling of the raw sequences using Phred software, the sequences are assembled using Phrap software (see Brent Ewing, LaDeana Hillier, Michael C. Wendl, and Phil Green. Base-calling of automated sequencer traces using phred. I. Accuracy assessment. 1998. Genome Research 8:175-185. and Brent Ewing and Phil Green Base-calling of automated sequencer traces using phred. II. Error probabilities. 1998. Genome Research 8:186-194). The assembly is reviewed using consed software. (See Consed: A Graphical Tool for Sequence Finishing Gordon et al 1998.) Criteria for completion are high quality, six-fold coverage of the entire full-length gene. The expected error rate per 10 kb of sequence should be&lt;0.1. If these criteria are not met, primers are selected along with templates for primer walking sequencing of the error-prone section of target DNA sequence. The primer walking sequencing is done on either the ABI 310 sequencer or through high-throughput sequencing using the ABI 3700 depending on volume of sequencing needed, and those sequences are subsequently added to the assembly. BLAST analysis is done for comparison especially to known genes. (See: Altschul, S. F., Gish, W., Miller, W., Myers, E. W. &amp; Lipman, D. J. (1990) “Basic local alignment search tool.” J. Mol. Biol. 215:403-410; Gish, W. &amp; States, D. J. (1993) “Identification of protein coding regions by database similarity search.” Nature Genet. 3:266-272; Madden, T. L., Tatusov, R. L. &amp; Zhang, J. (1996) “Applications of network BLAST server” Meth. Enzymol. 266:131-141; Altschul, S. F., Madden, T. L., Schäffer, A. A., Zhang, J., Zhang, Z., Miller, W. &amp; Lipman, D. J. (1997) “Gapped BLAST and PSI-BLAST: a new generation of protein database search programs.” Nucleic Acids Res. 25:3389-3402; and Zhang, J. &amp; Madden, T. L. (1997) “PowerBLAST: A new network BLAST application for interactive or automated sequence analysis and annotation.” Genome Res. 7:649-656.) The generated full-length sequence is imported into another assembly program called Sequencher. (See Cash, H., Clark, B., Galt, J., Garb, C., Goebel III, C. J., &amp; Singer, J.  Sequencher User Guide “The complete Software Solution for Sequencing DNA ”. Gene Codes Corporation. 1999.) With this program, it is easy to view the open reading frame to be sure mutations, if any, have not caused a frame shift. 
     It is to be understood that the foregoing examples are exemplary and explanatory only and are not restrictive of the invention. Various changes may be made to the embodiments described above by one of skill in the art without departing from the scope of the invention, as defined by the following claims.