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Optimization of PCRs 99 22. Saike, R. K., Gelfand, D. H., Stoffel, S., Scharf, S. J., Higuchi, R. Horu, G. T., Mullis, K. B., and Erlich, H. A. (1988) Primer-directed enzymatic amplification of DNA with a thermostable DNA polymerase. Science 239, 487– 491. 23. Flaman, J.-M., Frebourg, T., Moreau, V., Charbonnier, R., Martin, C., Ishioka, C., et al. (1994). A rapid PCR fidelity assay. Nucleic Acids Res. 22, 3259–3260. 24. Cline, J., Braman, J. C., and Hogrefe, H. H. (1996) PCR fidelity of Pfu DNA polymerase and other thermostable DNA polymerases. Nucleic Acids Res. 24, 3546–3551. 25. Sardelli, A. D. (1993) Plateau effect-understanding PCR limitations, in Amplifications: A Forum for PCR Users. Perkin–Elmer Corp., Norwald, CT, pp. 1. 26. Saiki, R. K. (1989) The design and optimization of the PCR, in PCR Technology (Erlich, H. A., ed.), Stockton Press, New York, pp. 7–16. 27. Kim, H. S. and Smithies, O. (1988) Recombinant fragment assay for gene targeting based on the polymerase chain reaction. Nucleic Acids Res. 16, 8887–8903. 28. McConlogue, L., Brow, M. D., and Innis, M. A. (1988) Structure-independent DNA amplification by PCR using 7-deaza-2′-deoxyguanosine. Nucleic Acids Res. 16, 9869. 29. Mytelka, D. S. and Chamberlin, M. J. (1996) Analysis and suppression of DNA polymerase pauses associated with a trinucleotide consensus. Nucleic Acids Res. 24, 2774–2781. 30. Pomp, D. and Medrano, J. F. (1991) Organic solvents as facilitators of polymerase chain reaction. BioTechniques 10, 58–59. 31. Newton, C. R. and Graham, A. (1994) PCR, Bios Scientific, Publishers Ltd., Oxford. 32. Levinson, G., Fields, R. A., Harton, G. L., Palmer, F. T., Maddleena, A., Fugger, E. F., et al. (1992) Reliable gender screening for human preimplantation embryos, using multiple DNA target-sequences. Hum. Reprod. 7, 1304–1313. 33. Chamberlain, J. S., Gibbs, R. A., Ranier, J. E., Nguyen, P. N., and Caskey, C. T. (1988) Deletion screening of the Duchenne muscular dystrophy locus via multiplex DNA amplification. Nucleic Acids Res. 16, 11,141–11,156. 34. Uggozoli, L. and Wallace, B. (1992) Application of an allele-specific polymerase chain reaction to the direct determination of ABO blood group genotypes. Genomics 12, 670–674. 35. Henke, W., Herdel, K., Jung, K., Schnorr, D., and Loening, S. A. (1997) Betaine improves the PCR amplification of GC-rich DNA sequences. Nucleic Acids Res. 25, 3957–3958. 36. Hengen, P. N. (1997) Optimizing multiplex and LA-PCR with betaine. Trends Biochem. Sci. 22, 225–226. 37. Bassam, B. J. and Caetano-Anolles, G. (1993) Automated “hot start” PCR using mineral oil and paraffin wax. BioTechniques 14, 30–34. 38. Wainwright, L. A. and Seifert, H. S. (1993) Paraffin beads can replace mineral oil as an evaporation barrier in PCR. BioTechniques 14, 34–36. 39. Rous, K. H. (1995) Optimization and troubleshooting in PCR, in PCR Primer (Diefferbach, C. W. and Dveksler, G. S. eds.), CSH Press, New York, pp. 53–62.
100 Grunenwald
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TM Methods in Molecular Biology Vol
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Xin Wang and W. Scott Young III 105
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63. Primed In Situ Nucleic Acid Lab
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4 Bartlett and Stirling The thing t
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6 Bartlett and Stirling Fig. 2. Res
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8 Carroll and Casimir of PCR. Such
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10 Carroll and Casimir cost more th
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12 Carroll and Casimir are no longe
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14 Carroll and Casimir Should these
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16 McDonagh Fig. 1. Unidirectional
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18 McDonagh stored. This means that
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20 McDonagh
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22 Stirling which will either not a
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24 Stirling
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28 Bartlett References 1. US Depart
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30 Bartlett and White 11. 5 M sodiu
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32 Bartlett and White
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34 Pearson and Stirling 11. Microfu
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36 Going 3. Methods 3.1. Section Cu
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38 Going pipet filler. Spread the p
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40 Going digitally to record the di
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42 Going
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44 Pearson 7. Add 60 µL of chlorof
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Page 49 and 50: 48 Pearson 3. Method The method of
Page 51 and 52: 50 Stirling and Bartlett 4. Protein
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Page 55 and 56: 54 Stirling 3. Methods 3.1. Fungal
Page 57 and 58: 56 McDonagh 2. Add 0.4 mL of TNE bu
Page 59 and 60: 58 Schmerer 2. Materials To apply t
Page 61 and 62: 60 Schmerer 3. The additional purif
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Page 67 and 68: 66 Bartlett Table 1 Recommended Aga
Page 69 and 70: 68 Bartlett Table 2 Separation of D
Page 71 and 72: 70 Bartlett 2. 5× TBE: 54 g of Tri
Page 73 and 74: 72 Bartlett 7. Remove upper aqueous
Page 75 and 76: 74 Bartlett 4. Many modern electrop
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Page 79 and 80: 78 Stirling 11. Store at -20°C for
Page 81 and 82: 82 Hyndman and Mitsuhashi 3.1. Effi
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Page 85 and 86: 86 Hyndman and Mitsuhashi Fig. 3. H
Page 87 and 88: 88 Hyndman and Mitsuhashi can be ge
Page 89 and 90: 90 Grunenwald may be affected by ea
Page 91 and 92: 92 Grunenwald 50°C will generally
Page 93 and 94: 94 Grunenwald of template DNA, a su
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Page 105 and 106: 106 Wang and Young full-length cDNA
Page 107 and 108: 108 Wang and Young Fig. 1. (A) Nort
Page 109 and 110: 110 Wang and Young Fig. 3. Expresse
Page 111 and 112: 112 Wang and Young 2. First-strand
Page 113 and 114: 114 Wang and Young 3′-RACE outlin
Page 115 and 116: 116 Wang and Young
Page 117 and 118: 118 Dassanayake and Samaranayake co
Page 119 and 120: 120 Dassanayake and Samaranayake 5.
Page 121 and 122: 122 Dassanayake and Samaranayake Re
Page 123 and 124: 124 Iannone et al. Fig. 1. Diagram
Page 125 and 126: Table 1 Oligonucleotides Descriptio
Page 127 and 128: 128 Iannone et al. 5. For microsphe
Page 129 and 130: 130 Iannone et al. 4. To adjust for
Page 131 and 132: 132 Iannone et al. 6. Target concen
Page 133 and 134: 134 Iannone et al.
Page 135 and 136: 136 Benjamin, Smith, and Waites amp
Page 137 and 138: 138 Benjamin, Smith, and Waites the
Page 139 and 140: 140 Benjamin, Smith, and Waites 2.2
Page 141 and 142: 142 Benjamin, Smith, and Waites 2.
Page 147 and 148: 148 Benjamin, Smith, and Waites 8.
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150 Benjamin, Smith, and Waites
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152 Olmos et al. Fig. 1. RT-hemines
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154 Olmos et al. This nested RT-PCR
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156 Olmos et al. Table 2 Volume and
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158 Olmos et al. 8. The sensitivity
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160 Olmos et al.
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162 Abe 5. Moloney murine leukemia
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164 Abe Table 2 Detection Rate of H
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166 Abe 4. For HBV, nested PCR usin
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168 Tellier et al. of Pfu (and ther
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170 Tellier et al. 2. Cline, J., Br
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172 Tellier et al. 38. Tamiya, S.,
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174 Tellier et al. 13. Thin-wall PC
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176 Tellier et al. 13 min for the l
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178 Tellier et al.
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182 Stirling efficiency of the reac
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184 Stirling
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186 Cremer and Moos Fig. 1. Rearran
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188 Cremer and Moos 4. Count cells
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190 Cremer and Moos Fig. 3. Alignme
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192 Cremer and Moos Fig. 4. Testing
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194 Cremer and Moos 5. Compare the
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196 Cremer and Moos 11. Klein, E.,
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198 McDonagh the dilution method is
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200 McDonagh 2.2. Basic PCR 1. dNTP
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202 McDonagh Fig. 2. Quantitative P
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204 McDonagh
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206 Bartlett Table 1 Example Assay
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208 Bartlett 3.4. Calculation of Re
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210 Bartlett 11. Cerenkov counting
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212 Kerr Fig. 1. Fluorescent probes
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214 Kerr after the PCR. This reduce
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218 Bartlett As with any experiment
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220 Bartlett Even once novel regula
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222 Bartlett Notwithstanding these
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224 Bartlett
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226 Dominguez et al. Table 1 Primer
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228 Dominguez et al. 4. Oligonucleo
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230 Dominguez et al. Fig. 2. cDNA n
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232 Dominguez et al. 3.4. Gel Elect
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234 Dominguez et al. 3. If the cont
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236 Dominguez et al. 11. Joshi, C.
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238 Khalturin, Kuznetsov, and Bosch
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246 Ringquist et al. In this chapte
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248 Ringquist et al. 5. Total RNA s
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250 Ringquist et al. 3. Purificatio
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252 Ringquist et al. 2. The present
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254 Ringquist et al.
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256 Case-Green, Pritchard, and Sout
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272 Oien Fig. 1. A schematic diagra
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274 Oien 4. 100% and 70% ethanol. 5
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276 Oien 2. Purify polyA + mRNA fro
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278 Oien 50-mL conical tubes. Resus
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280 Oien Forward Primer, and then r
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282 Oien 8. PCR. With SAGE, achievi
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284 Oien
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288 Edwards and Bartlett technology
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290 Edwards and Bartlett ing less p
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292 Edwards and Bartlett Stepwise m
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294 Edwards and Bartlett
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296 Rithidech and Dunn 11. Ethidium
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298 Rithidech and Dunn Fig. 1. PCR
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300 Rithidech and Dunn
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302 Edwards and Bartlett Studies th
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304 Edwards and Bartlett 11. Hot st
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306 Edwards and Bartlett Fig. 1. Ex
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308 Edwards and Bartlett 3. Sartor,
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310 Schmerer the investigation conc
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312 Schmerer References 1. Kunkel,
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314 Schmerer
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316 Aubele and Smida 2.2. Chemicals
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318 Aubele and Smida References 1.
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320 Nakashima, Akahoshi, and Tanaka
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322 Nakashima, Akahoshi, and Tanaka
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324 Stirling 9. TAE (20×): 484 g o
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326 Stirling
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328 Han and Robinson Fig. 1. Basic
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330 Han and Robinson sequence diffe
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332 Han and Robinson 4. Notes 1. PC
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334 Han and Robinson
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338 Stirling of simple and improved
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340 Stirling concentrations interfe
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342 Daniels to sequence a 500-bp PC
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344 Daniels 4. Load all of the samp
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346 Daniels References 1. Orita, M.
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348 Kösel et al. Fig. 1. Schematic
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350 Kösel et al. 3. Methods 3.1. P
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352 Kösel et al. Fig. 2. Sequencin
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354 Kösel et al. 5. Kwok, S. and H
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356 Mazars and Theillet Fig. 1. Sch
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358 Mazars and Theillet of genomic
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360 Mazars and Theillet
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362 Suomalainen and Syvänen Fig. 1
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364 Suomalainen and Syvänen detect
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366 Suomalainen and Syvänen temper
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368 Shen et al. ladder. Also, direc
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370 Shen et al. 3. Mineral oil. 4.
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372 Shen et al. extended primers, w
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374 Quivy and Becker Fig. 1. The us
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376 Quivy and Becker that decreases
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378 Quivy and Becker 2. Solution of
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380 Quivy and Becker 7. Precipitate
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382 Quivy and Becker 7. Prepare a p
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384 Quivy and Becker
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386 Walsh by most, but not all M13
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388 Walsh PCR products are now flus
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390 Walsh 5. For palindromic restri
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392 Walsh
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394 McAleer, Coffey, and Dunham Fig
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396 McAleer, Coffey, and Dunham Tab
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398 McAleer, Coffey, and Dunham Tab
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400 McAleer, Coffey, and Dunham
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402 Stirling 5. Homopolymer Regions
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406 Speel, Ramaekers, and Hopman Ta
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408 Speel, Ramaekers, and Hopman Fi
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410 Speel, Ramaekers, and Hopman po
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Table 2 Comparison of PRINS, in Sit
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414 Speel, Ramaekers, and Hopman te
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Table 3 Summary of Control Experime
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418 Speel, Ramaekers, and Hopman 3.
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420 Speel, Ramaekers, and Hopman ad
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422 Speel, Ramaekers, and Hopman 25
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426 Bull and Paskins Fig. 1. Result
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428 Bull and Paskins 2.3. Detection
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430 Bull and Paskins 6. Shake the s
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432 Bull and Paskins
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434 Wiedorn and Goldmann Fig. 1. IS
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436 Wiedorn and Goldmann 41. Protei
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438 Wiedorn and Goldmann 2. Incubat
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440 Wiedorn and Goldmann 3.15. Prim
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442 Wiedorn and Goldmann ficient se
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444 Wiedorn and Goldmann 25. Kommin
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446 Gilchrist and Befus Fig. 1. Sch
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448 Gilchrist and Befus 2. Cells ar
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450 Gilchrist and Befus Fig. 3. RT
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452 Gilchrist and Befus References
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454 Speel, Ramaekers, and Hopman of
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456 Speel, Ramaekers, and Hopman Fi
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462 Speel, Ramaekers, and Hopman bu
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468 Pearson and Stirling into PCR p
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470 Wang 2. Materials 2.1. PCR 1. D
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472 Wang Fig. 1. A brief outline of
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474 Wang
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476 Horton, Raju, and Conti-Fine Fi
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478 Horton, Raju, and Conti-Fine th
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480 Horton, Raju, and Conti-Fine 1.
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482 Horton, Raju, and Conti-Fine ot
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484 Horton, Raju, and Conti-Fine
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486 Preston amplification approach
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488 Preston 1. 10× PCR buffer: 100
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490 Preston Fig. 1. Design of degen
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492 Preston 2. Remove the AmpliTaq
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494 Preston 3.3. Cloning and DNA Se
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496 Preston MgCl 2 concentrations b
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498 Preston 21. Hung, T., Mak, K.,
Page 487 and 488:
500 Ravassard et al. Fig. 1. Constr
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502 Ravassard et al. size dispersio
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504 Ravassard et al. 9. ddH 2 O. 10
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506 Ravassard et al. 3.2.2. RNA Mix
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508 Ravassard et al. 4. Wash twice
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510 Ravassard et al.
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512 Pont-Kingdon Fig. 1. Constructi
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514 Pont-Kingdon 9. Invert tube and
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516 Pont-Kingdon
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518 Jones and Winistorfer Fig. 1. D
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520 Jones and Winistorfer Fig. 2. D
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522 Jones and Winistorfer The yield
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524 Jones and Winistorfer 7. Goulde
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526 Burke and Barik Fig. 1. The bas
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528 Burke and Barik concentration o
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530 Burke and Barik purified mutant
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532 Burke and Barik
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