DNA binding specificity and sequence of Xanthomonas campestris catabolite gene activator protein-like protein

Dong, Qianping; Ebright, Richard H.

doi:10.1128/jb.174.16.5457-5461.1992

Cited by 34 publications

(30 citation statements)

References 31 publications

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“…Using mutant sequences of the E. coli lac promoter as substrates, Clp has been shown to have the same DNA-binding specificity as CRP at positions 5, 6 and 7 (GTG motif) of the DNA half-site (Dong & Ebright, 1992). In our previous studies with the Xcc engA promoter, site-directed mutagenesis also indicated that the GTG motif of the proposed Clp core consensus sequence is essential for both DNA-protein complex formation in vitro and engA gene expression in vivo (Hsiao et al, 2005).…”

Section: Resultsmentioning

confidence: 99%

Regulation of the pehA gene encoding the major polygalacturonase of Xanthomonas campestris by Clp and RpfF

Hsiao

Zheng

et al. 2008

Microbiology

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Exopolysaccharide and several extracellular enzymes of Xanthomonas campestris pv. campestris (Xcc), the causative agent of black rot in crucifers, are virulence factors. In this study, sequence and mutational analysis has demonstrated that Xcc pehA encodes the major polygalacturonase, a member of family 28 of the glycosyl hydrolases. Using the 59 RACE (rapid amplification of cDNA ends) method, the pehA transcription initiation site was mapped at 102 nt downstream of a Clp (cAMP receptor protein-like protein)-binding site. Transcriptional fusion assays showed that pehA transcription is greatly induced by polygalacturonic acid, positively regulated by Clp and RpfF (an enoyl-CoA hydratase homologue which is required for the synthesis of cis-11-methyl-2-dodecenoic acid, a low-molecular-mass diffusible signal factor), subjected to catabolite repression, which is independent of Clp or RpfF, and repressed under conditions of oxygen limitation or nitrogen starvation. Our findings extend previous work on Clp and RpfF regulation to show that they both influence the expression of pehA in Xcc.

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Section: Resultsmentioning

confidence: 99%

Regulation of the pehA gene encoding the major polygalacturonase of Xanthomonas campestris by Clp and RpfF

Hsiao

Zheng

et al. 2008

Microbiology

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“…Using mutant sequences of the E. coli lac promoter as the substrates, the X. campestris Clp has been shown to have the same DNA binding specificity as CRP at positions 5, 6, and 7 (GTG motif) of the DNA half site [26]. Two consensus Clp-binding sites with a spacer of 27 nt were present at nt À80 to À59 (site I, centered at À69.5) and À53 to À32 (site II, centered at À42.5) relative to TIS (Fig.…”

Section: The Enga Upstream Region Possesses Two Clp-binding Sitesmentioning

confidence: 99%

“…engA promoter resembles class II CRP-dependent promoter except the presence of tandem Clp sites and a much shorter spacer than those of tandem CRP sites The amino acid residues that contact DNA base pairs in CRP-DNA complex are R180 and E181 in CRP, which are conserved in Clp, R201 and E202 [26]. The residues (A156, M157, T158, H159, P160, D161, and G162) in CRP making direct protein-protein interaction with the E. coli RNA polymerase a subunit C-terminal domain (aCTD) in transcription activation are also highly conserved in Clp (A177, M178, S179, H180, P181, Q182, and G183) [26,28,29]. The amino acids similar to the region in E. coli RNA polymerase aCTD (T285, E286, V287, E288, L289, G315, R317 and L318) responsible for interaction with CRP are also found in the X. campestris RNA polymerase aCTD (T284, E285, V286, E287, L288, G314, K316 and L317) [26,28,29].…”

Section: 7mentioning

confidence: 99%

“…The residues (A156, M157, T158, H159, P160, D161, and G162) in CRP making direct protein-protein interaction with the E. coli RNA polymerase a subunit C-terminal domain (aCTD) in transcription activation are also highly conserved in Clp (A177, M178, S179, H180, P181, Q182, and G183) [26,28,29]. The amino acids similar to the region in E. coli RNA polymerase aCTD (T285, E286, V287, E288, L289, G315, R317 and L318) responsible for interaction with CRP are also found in the X. campestris RNA polymerase aCTD (T284, E285, V286, E287, L288, G314, K316 and L317) [26,28,29]. With such conservations, it is likely that equivalent amino acids of CRP and Clp make equivalent contacts in the respective proteinpromoter complexes and direct protein-protein interactions with the RNA polymerase in transcription activation.…”

Section: 7mentioning

confidence: 99%

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Clp upregulates transcription of engA gene encoding a virulence factor in Xanthomonas campestris by direct binding to the upstream tandem Clp sites

Hsiao¹,

Liao

Lee³

et al. 2005

FEBS Letters

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In Xanthomonas campestris, the causative agent of black rot in crucifers, the endoglucanase level is greatly decreased in the mutant deficient in Clp, a homologue of cyclic AMP receptor protein (CRP). It is established that Clp has the same DNA binding specificity as CRP at positions 5, 6, and 7 (GTG motif) of the DNA half site. In this study, the engA transcription initiation site was determined by the 5 0 RACE method, and two consensus Clp-binding sites, site I and site II centered at À69.5 and À42.5, respectively, were located. Transcriptional fusion assays indicated that Clp greatly activates engA transcription. Site-directed mutagenesis indicated that position 5 of GTG motif in site II is essential for both DNA-protein complex formation in electrophoretic mobility shift assays and engA transcription in vivo. In addition, mutation at position 5 of site I drastically reduces the promoter activity, indicating that binding of Clp to site I exerts a synergistic effect on the transcription activation by site II. engA appears to be the first X. campestris gene known to be activated by Clp via a direct binding to the promoter.

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“…Data represent means ± SD of three experiments engXCA promoter [9]. The DNA sequence for Clp binding has been evaluated and found to be similar to that of the E. coli CRP-binding site (5 0 -AAATGTGA-TCTAGA-TCACATTT-3 0 ) [4]. This binding site is 22 bp in length and exhibits perfect twofold sequence symmetry, with the bold-type bases representing the left and right sites each for the binding of one subunit of the active CRP dimer [15].…”

Section: Clp Regulated Transcription Of Xpse Gene Through Directly Bimentioning

confidence: 99%

Regulation of the Type II Secretion Structural Gene xpsE in Xanthomonas campestris Pathovar campestris by the Global Transcription Regulator Clp

2008

Curr Microbiol

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DNA binding specificity and sequence of Xanthomonas campestris catabolite gene activator protein-like protein

Cited by 34 publications

References 31 publications

Regulation of the pehA gene encoding the major polygalacturonase of Xanthomonas campestris by Clp and RpfF

Regulation of the pehA gene encoding the major polygalacturonase of Xanthomonas campestris by Clp and RpfF

Clp upregulates transcription of engA gene encoding a virulence factor in Xanthomonas campestris by direct binding to the upstream tandem Clp sites

Regulation of the Type II Secretion Structural Gene xpsE in Xanthomonas campestris Pathovar campestris by the Global Transcription Regulator Clp

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