laboratory: unit 3: purify pcr product (55-65) lecture: dna sequencing in-class writing: discuss...
TRANSCRIPT
Laboratory: Unit 3: purify PCR product (55-65)
Lecture: DNA sequencing
In-Class Writing: discuss abstracts (pages 68, 157) & AEM 63: 2647-53, 1997
Hand In: nothing Read: sample problems (pages 135-150)
Due Next Class: nothing
Dye Primer Sequencing
Dye Terminator Sequencing
Enterococcus faecium
Enterococcus faecium
Lactobacillus paracasei
Sequence polymorphism in Lactobacillus paracasei 16S rRNA genes
mixed template
mixed template
DNA Preparation for Sequencing
DNA must be free of contaminants.
Submit samples in dH2O or Tris, not Tris/EDTA.
DNA Preparation for Sequencing
Remove unincorporated dNTPs & primers (Qiagen kit).
10 µL of DNA/reaction @ 50 ng/uL = 500 ng of amplicon in 10 L
DNA Preparation for Sequencing
Estimate PCR product concentration by agarose gel electrophoresis.
Compare to DNA Mass Ladder.
DNA Preparation for Sequencing
Difficult to estimate PCR product concentration with conventional spectrophotometer.
Use nanodrop spectrophotometer to estimate DNA concentration.
Sequencing Primers
Primers (10 µL/reaction) @ 10 µM = 10 pmol/µL
= 61.6 ng/L for 8-27F primer (MW = 6161)
Tips for Primer Design
18-22 bases long GC content = 50-60%
Annealing temperature 50-65oC.
Avoid 3 identical contiguous bases.
Sequencing tandem repeats difficult. Primers should not anneal near repeats.
Purify PCR product prior to sequencing
binding buffer (PB) = high salt
wash buffer (PE) = high salt + ethanol
Purify PCR product prior to sequencing
50 ul distilled water
dissolve in 50 ul distilled water
ready for sequencing
Use a yellow tip to remove drops of ethanol trapped on the rim above the filter before you elute the DNAwith water.
Low Mass Ladder(Invitrogen)
ng:200
120
80
40
20
(10)
bp:2000
1200
800
400
200
(100)
2% 3:1 agarose gel
Although the Amazon Basin is well known for its diversity of flora and fauna, this report represents the first description of the microbial diversity in Amazonian soils involving a culture-independent approach. Among the 100 sequences of genes coding for small-subunit rRNA obtained by PCR amplification with universal small-subunit rRNA primers, 98 were bacterial and 2 were archaeal. No duplicate sequences were found, and none of the sequences had been previously described. Eighteen percent of the bacterial sequences could not be classified in any known bacterial kingdom. Two sequences may represent a unique branch between the vast majority of bacteria and the deeply branching, predominantly thermophilic bacteria. Five sequences formed a clade that may represent a novel group within the class Proteobacteria. In addition, rRNA intergenic spacer analysis was used to show significant microbial population differences between a mature forest soil and an adjacent pasture soil.