Primers used for MLST of Campylobacter lari

Genes

The Campylobacter lari MLST scheme uses internal fragments of the following seven house-keeping genes:

adk (adenylate kinase)
atpA (ATP synthase alpha subunit)
glnA (glutamine synthetase)
glyA (serine hydroxy methyl transferase)
pgi (glucose-6-phosphate isomerase)
pgm (phospho glucomutase)
tkt (transketolase)

PCR Amplification and sequencing

The primer pairs used for the PCR amplification and sequencing are detailed below:

adk
Forward
adkF: TGAAAGAATTRTTTTTAATCATAGG
Reverse
adkR: CTTTCATRTCWGCHACGATAGGTTC

atpA
Forward
atpAF: GWCAAGGDGTTATYTGTATWTATGTTGC
Reverse
atpAR: TTTAADAVYTCAACCATTCTTTGTCC

glnA
Forward
glnAF: TGATAGGMACTTGGCAYCATATYAC
Reverse
glnAR: ARRCTCATATGMACATGCATACCA

glyA
Forward
glyAF: ATTCAGGTTCTCAAGCTAATCAAGG
Reverse
glyAR: GCTAAATCYGCATCTTTKCCRCTAAA

pgi
Forward
pgiF1: TAGTGGGWATGGGAGGDTCAAGTT
Reverse
pgiR1: CCAATDAGWGCDATAGGAGTTAAACC

pgm
Forward
pgmF3: CGTGTTGTTTTAGATGTGGCTCA
Reverse
pgmR3: ATAGCGAAACAAACTAGCAATTCCT

tkt
Forward
tktF2: GCCTTTGGGTTTAGCRGATATTATG
Reverse
tktR: TTTTAATHAVHTCTTCRCCCAAAGGT

Reaction conditions - PCR

Denaturation: 94ºC 30 s
Annealing: 53ºC 30 s
Extension: 72ºC 2 minutes
30 cycles

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Citing the database

The preferred format for citing this website in publications is:

This publication made use of the Campylobacter lari MLST website (http://pubmlst.org/ clari/) developed by Keith Jolley and sited at the University of Oxford (Jolley et al. 2004, BMC Bioinformatics, 5:86). The development of this site has been funded by the Wellcome Trust.

Related databases

C. fetus
C. jejuni (and C. coli)
C. helveticus
C. insulaenigrae
C. upsaliensis

Status

Profile database

Profiles: 18
Last updated: 2008-02-20

Isolate database

Isolates: 19
Last updated: 2004-11-10