Download Table S3.

Table S3. Oligonucleotides used in this study.
PCR target
Sequence (5’-3’)
Forward and reverse primer
(a) Primers for PhoB-3xFLAG expressing strain (MG1655_PhoB_FLAG)
phoB and pSUB11
5’-GACCGTGCGCGGTACAGGATATCGTTTTTCA
phoB-pSUB11-F
ACCCGCTTTGACTACAAAGACCATGACGG-3’
5’-ATAAGCCCTGCTCTGCGTCCGATGAGCAAGG
phoB-pSUB11-R
CGTTAAAAGCATATGAATATCCTCCTTAG-3’
phoB
phoB-check1122-F
5’-TGCCAGTCTGAGGTGTGAAG-3’
phoB-check1122-R
5’-GGCGCAATAAATTCCAGAAA-3’
(b) Primers for detection of inserts of pGL3 derivatives
pGL3-basic vector
pGL3_InsChk_F
5’-GGTACGGGAGGTACTTGGAGC-3’
pGL3_InsChK_R
5’-GGCCTTTCTTTATGTTTTTGGC-3’
(c) Primers for constructing PhoB-His fusion protein expressing vector
phoB
PhoB_His_F
5’-GCCCATGGCGAGACGTATTCTGGTCG-3’
PhoB_His_R
5’-GCAAGCTTAAAGCGGGTTGAAAAACGATATCCTG-3’
(d) Primers for constructing promoter::luciferase fusionsa
phoB
cusC
cusR
feaR
mipA
prpR
sbcD
ydfH
yedX
yegH
phoB_FPB
5’-GCGCTAGCACGGTAGTATTGAGGAACGCC-3’
phoB_RPB
5’-GCCCATGGGATTTGCCCTGTTGTAATAAATAGG-3’
cusC_FPB
5’-GCGCTAGCCGCCAGCAGTTCAGCAAA
cusC_RPB
5’-GCCCATGGAGGCTCATAATTTCTGGTGATTTTA
cusR_FPB
5’-GCGCTAGCTTAAGATTACCGCTCCAGCTGC
cusR_RPB
5’-GCCCATGGATTTCCTCCGCATGTTGCC
feaR_FPB
5’-GCGCTAGCGTAGCAGAATACGTTCACGCTCTG
feaR_RPB
5’-GCCCATGGGGCACGTTTTCGCTCTGT
mipA_FPB
5’-GCGCTAGCTGCAGTGTGAACTCTTCGTCCT
mipA_RPB
5’-GCCCATGGAATTAATCATTCCTTAAACAAATGTTTAG
prpR_FPB
5’-GCGCTAGCTATCCGCATCCACCAGCA
prpR_RPB
5’-GCCCATGGAGCGCACCGCAAAGTTAAG
sbcD_FPB
5’-GCGCTAGCTGATATAGTCATCCGCGCCG
sbcD_RPB
5’-GCCCATGGAACGGTTCCCTGGCGAAA
ydfH_FPB
5’-GCGCTAGCCGCCGTCTTACCGGGTATG
ydfH_RPB
5’-GCCCATGGTCGTTCTTGCTTGTGAGTGAGTTAA
yedX_FPB
5’-GCGCTAGCGAATTCAAAGCGTGATGTTGC
yedX_RPB
5’-GCCCATGGGTTTATATCCTTGTCATGTGAATGAGT
yegH_FPB
5’-GCGCTAGCTGGTCTTTCAGGCATCCAGA
yegH_RPB
5’-GCCCATGGAGTAAGTACAAAACCTATTCGTTGTATGA
yhjC
yhjC_FPB
5’-GCGCTAGCAAAGACTTAAGTAGTGGAAGGGTATTACC
yhjC_RPB
5’-GCCCATGGTTCTTTGACCGATTGTTGTTCAC
(e) Oligonucleotidesb for DNA binding assay
mipA
5’-GCGTTACTGGCGAGCCTGGTCTTTACATT
mipA_p
AATTATGCAAAATTTATGGATGAGTTGTTGA-3’
5’-TCAACAACTCATCCATAAATTTTGCATAAT
mipA_c
TAATGTAAAGACCAGGCTCGCCAGTAACGC-3’
yedX
5’-ATGTTATAGAAACAGCCTGGTTCATTACAA
yedX_p
AATTGTAATGCTGCTGTAAGGTTACCCTGG-3’
5’-CCAGGGTAACCTTACAGCAGCATTACAAT
yedX_c
TTTGTAATGAACCAGGCTGTTTCTATAACAT-3’
ydfH
5’-GCGTAACTGCCGGGTTATTGCTTGTCACA
ydfH_p
AAAAAGTGGTAGACTCATGCAGTTAACTCAC-3’
5’-GTGAGTTAACTGCATGAGTCTACCACTTT
ydfH_c
TTTGTGACAAGCAATAACCCGGCAGTTACGC-3’
cusR
5’-TGGCAATCGCTTATTGGCAAAATGACAAT
cusR_p
TTTGTCATTTTTCTGTCACCGGAAAATCAGA-3’
5’-TCTGATTTTCCGGTGACAGAAAAATGACA
cusR_c
AAATTGTCATTTTGCCAATAAGCGATTGCCA-3’
yhjC
5’-TGAGAAATCGCCACATTCGGCATGACAAC
yhjC_p
ATTGTGAAACCCGGCATTAGATGTTAGAAAA-3’
5’-TTTTCTAACATCTAATGCCGGGTTTCACAA
yhjC_c
TGTTGTCATGCCGAATGTGGCGATTTCTCA-3’
yegH
5’-CGATTTATCCATGATCGAATTGTGACATTT
yegH_p
GTCATACAACGAATAGGTTTTGTACTTACT-3’
5’-AGTAAGTACAAAACCTATTCGTTGTATGAC
yegH_c
AAATGTCACAATTCGATCATGGATAAATCG-3’
feaR
5’-TCTGTGAAATGTATTTTTATTGTTGCATTT
feaR_p
GTGTTGCAATAAACGAAGCTAATGAGCCTG-3’
5’-CAGGCTCATTAGCTTCGTTTATTGCAACA
feaR_c
CAAATGCAACAATAAAAATACATTTCACAGA-3’
prpR
5’-CCGAATATTGGGTTTAGTCTTGTTTCATAA
prpR_p
TTGTTGCAATGAAACGCGGTGAAACATTGC-3’
5’-GCAATGTTTCACCGCGTTTCATTGCAACA
prpR_c
ATTATGAAACAAGACTAAACCCAATATTCGG-3’
yahA
5’-TATCCGCCACGGGGAGTAATAGTCACAGA
yahA_p
TATATTAATGATAATCACTATCACCATATCG-3’
5’-CGATATGGTGATAGTGATTATCATTAATATA
yahA_c
TCTGTGACTATTACTCCCCGTGGCGGATA-3’
cof
5’-GTTTTCGTTATCAGATAATCGATGTCAAAA
cof_p
AAATGCCACTCGGCAGCGTCACCAAGATCT-3’
5’-AGATCTTGGTGACGCTGCCGAGTGGCATT
cof_c
TTTTTGACATCGATTATCTGATAACGAAAAC-3’
yddV
5’-TTGCGATACGGTATTTCTTATCTGTAATAAA
yddV_p
AATTTCACCCGCAGACTTCTGTTATTCAA-3’
5’-TTGAATAACAGAAGTCTGCGGGTGAAATT
yddV_c
TTTATTACAGATAAGAAATACCGTATCGCAA-3’
a
For the construction of pGL3 derivative plasmids, the upstream region was around
500 bps in front of the translation start site of each gene.
b
For each binding candidate, complimentary oligonucleotide of 60 base pairs centered
at the corresponding putative binding site were first end-labeled with biotin separately
and then annealed before use.