A genetic screen identifies genes and sites involved in pilin antigenic variation in <i>Neisseria gonorrhoeae</i>

Sechman, Eric V.; Rohrer, Melissa S.; Seifert, H. Steven

doi:10.1111/j.1365-2958.2005.04657.x

Cited by 68 publications

(158 citation statements)

References 61 publications

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“…We insertionally inactivated the nlpD gene by inserting a cat resistance gene cassette in place of the coding sequence. The strain FA1090 nv (the subscript "nv" in the strain name indicates that a strain cannot undergo pilin antigenic variation [24]) used in this study contained either 1-81-S2 or RM11.2 pilE variant sequences. Each of the FA1090 variants were transformed with the mutant ⌬nlpD::cat allele construct (here designated ⌬nlpD) by spot transformation, and Cam r colonies were selected on Cam plates.…”

Section: Genetic Analysis Of the Nlpd Ortholog Of Neisseria Gonorrhoeaementioning

confidence: 99%

The Gonococcal NlpD Protein Facilitates Cell Separation by Activating Peptidoglycan Cleavage by AmiC

et al. 2016

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Key steps in bacterial cell division are the synthesis and subsequent hydrolysis of septal peptidoglycan (PG), which allow efficient separation of daughter cells. Extensive studies in the Gram-negative, rod-shaped bacterium Escherichia coli have revealed that this hydrolysis is highly regulated spatially and temporally. Neisseria gonorrhoeae is an obligate Gram-negative, diplococcal pathogen and is the only causative agent of the sexually transmitted infection gonorrhea. We investigated how cell separation proceeds in this diplococcal organism. We demonstrated that deletion of the nlpD gene in strain FA1090 leads to poor growth and to an altered colony and cell morphology. An isopropyl-beta-D-galactopyranoside (IPTG)-regulated nlpD complemented construct can restore these defects only when IPTG is supplied in the growth medium. Thin-section transmission electron microscopy (TEM) revealed that the nlpD mutant strain grew in large clumps containing live and dead bacteria, which was consistent with deficient cell separation. Biochemical analyses of purified NlpD protein showed that it was able to bind purified PG. Finally, we showed that, although NlpD has no hydrolase activity itself, NlpD potentiates the hydrolytic activity of AmiC. These results indicate that N. gonorrhoeae NlpD is required for proper cell growth and division through its interactions with the amidase AmiC. IMPORTANCE N. gonorrhoeae is the sole causative agent of the sexually transmitted infection gonorrhea. The incidence of antibiotic-resistant gonococcal infections has risen sharply in recent years, and N. gonorrhoeae has been classified as a "superbug" by the CDC. Since there is a dearth of new antibiotics to combat gonococcal infections, elucidating the essential cellular process of N. gonorrhoeae may point to new targets for antimicrobial therapies. Cell division and separation is one such essential process. We identified and characterized the gonococcal nlpD gene and showed that it is essential for cell separation. In contrast to other pathogenic bacteria, the gonococcal system is streamlined and does not appear to have any redundancies.

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Section: Genetic Analysis Of the Nlpd Ortholog Of Neisseria Gonorrhoeaementioning

confidence: 99%

The Gonococcal NlpD Protein Facilitates Cell Separation by Activating Peptidoglycan Cleavage by AmiC

et al. 2016

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“…During pilin antigenic variation, a variable portion of a pilS copy replaces the corresponding portion of pilE, recombining at short regions of identity shared between the silent and expressed genes (16). Pilin antigenic variation is dependent on recA (21), the recF-like pathway (33,57), rdgC (32), and rep (19) as well as the ruvABC and recG branch migration pathways (50).…”

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confidence: 99%

“…Recombinational repair is well studied in N. gonorrhoeae and requires the recA (21) and recX (62) genes, along with either the RecBCD pathway components recB, recC, and recD (33) or the RecF pathway components recO, recR, recQ, and recJ (33,50,57). The branch migration genes recG and ruvA also contribute to recombinational DNA repair in N. gonorrhoeae (50). The use of multiple genetic pathways for recombinational DNA repair in N. gonorrhoeae distinguishes it from Escherichia coli, which utilizes the RecF DNA repair pathway only in a mutant recBC sbcBC background (22,25).…”

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Mutation of the priA Gene of Neisseria gonorrhoeae Affects DNA Transformation and DNA Repair

Kline

Seifert

2005

J Bacteriol

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In Escherichia coli, PriA is central to the restart of chromosomal replication when replication fork progression is disrupted and is also involved in homologous recombination and DNA repair. To investigate the role of PriA in recombination and repair in Neisseria gonorrhoeae, we identified, cloned, and insertionally inactivated the gonococcal priA homologue. The priA mutant showed a growth deficiency and decreased DNA repair capability and was completely for deficient in DNA transformation compared to the isogenic parental strain. The priA mutant was also more sensitive to the oxidative damaging agents H 2 O 2 and cumene hydroperoxide compared to the parental strain. These phenotypes were complemented by supplying a functional copy of priA elsewhere in the chromosome. The N. gonorrhoeae priA mutant showed no alteration in the frequency of pilin antigenic variation. We conclude that PriA participates in DNA repair and DNA transformation processes but not in pilin antigenic variation.

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“…Pilin variation was measured using the previously described pilus-dependent colony morphology changes (PDCMC) assay (Sechman et al, 2005), which monitors formation of faster-growing P À colony outgrowths that emerge on the edge of P + colonies over time with the following modifications. P + and P À colonies vary morphologically and are indicative of pilus expression.…”

Section: Methodsmentioning

confidence: 99%

“…To test this, we measured pilin variation of the dprA mutants using a colony morphology proxy for pilin variation. PDCMC, which are indicative of pilin variation (Sechman et al, 2005), were measured and quantified in our strains. Cells lacking functional DprA exhibited significantly higher pilin variation compared to parental cells in both FA1090 and MS11 (P<0.05, Fig.…”

Section: Dpra Affects Pilin Variationmentioning

confidence: 99%

DprA is required for natural transformation and affects pilin variation in Neisseria gonorrhoeae

Duffin

Barber

2016

Microbiology

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Natural transformation is the main means of horizontal genetic exchange in the obligate human pathogen Neisseria gonorrhoeae and drives the spread of antibiotic resistance and virulence determinants. Transformation can be divided into four steps: (1) DNA binding, (2) DNA uptake, (3) DNA processing and (4) DNA recombination into the chromosome. The DNA processing enzyme DprA has been shown to shuttle incoming ssDNA to the recombination enzyme RecA during transformation in Bacillus subtilis and Streptococcus pneumoniae. Here, we investigate the role of DprA during transformation in N. gonorrhoeae. Inactivation of dprA completely abrogated transformation of gyrB1-encoding DNA, which confers nalidixic acid resistance. The presence of the DNA uptake sequence enhances DNA uptake and transformation by binding to the minor pilus protein ComP. Loss of transformation in the dprA null mutants was independent of the DNA uptake sequence. DprA mutants exhibited increased RecA-dependent pilin variation suggesting that DprA affects pilin variation. Unlike the exquisite UV sensitivity of a recA mutant, inactivation of dprA did not affect survival following UV irradiation. These results demonstrate that DprA has a conserved function during transformation, and reveal additional effects of DprA in N. gonorrhoeae during pilin variation.

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A genetic screen identifies genes and sites involved in pilin antigenic variation in Neisseria gonorrhoeae

Cited by 68 publications

References 61 publications

The Gonococcal NlpD Protein Facilitates Cell Separation by Activating Peptidoglycan Cleavage by AmiC

The Gonococcal NlpD Protein Facilitates Cell Separation by Activating Peptidoglycan Cleavage by AmiC

Mutation of the priA Gene of Neisseria gonorrhoeae Affects DNA Transformation and DNA Repair

DprA is required for natural transformation and affects pilin variation in Neisseria gonorrhoeae

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