Characterization of Fifty Putative Inclusion Membrane Proteins Encoded in the<i>Chlamydia trachomatis</i>Genome

Li, Zhongyu; Chen, Chaoqun; Ding, Chan; Wu, Yimou; Zhong, Youmin; Zhong, Guangming

doi:10.1128/iai.00010-08

Cited by 133 publications

(165 citation statements)

References 61 publications

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“…GST-fusion recombinant proteins of D111, D628, D622, D702, D509, and D694 were expressed in a pGEX expression system (GST was fused to the N terminus of the chlamydial proteins) and purified by glutathione-conjugated agarose beads (Amersham Biosciences, Pittsburgh, USA) as described previously [41][42][43]. To monitor the processing of chlamydia T cell antigens by CPAF, a cell-free pre-incubation assay was used as described elsewhere [36].…”

Section: Cell-free Degradation Assay and Coomassie Blue Stainingmentioning

confidence: 99%

CPAF selectively degrades chlamydial T cell antigens for inhibiting antigen presentation

Zhang

Zhong

Cai

et al. 2017

J Infect Dev Ctries

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Introduction: Chlamydia trachomatis is the leading cause of sexually transmitted bacterial disease, which may cause significant threats, such as pelvic inflammatory disease and tubal factor infertility, to women if untreated. The pathological mechanisms of chlamydia-induced disease remain largely unknown, but it has been proposed that CPAF, a chlamydia-secreted serine protease, may play major roles in aiding chlamydial infection and contribute to chlamydia pathogenesis during in vivo infection. According to previous results, CPAF targets host immunity by degrading antimicrobial peptides and neutralizing complement activity; however, whether CPAF is involved in chlamydial antigen presentation has never been reported. Methodology: Antigen presentation assay was used to monitor the effects of CPAF on OT1-, OT2-, and chlamydia T cell antigen-mediated antigen presentation. In vitro cell-free degradation assay was used to detect CPAF processing of chlamydia T cell antigens. Results: We found that CPAF preferably inhibits OT2-but not OT1-mediated antigen presentation. CPAF inhibits OT2 antigen presentation by direct proteolytic cleavage in the wild type CPAF, but not enzymatic mutants. Importantly, several previously identified chlamydial T cell antigens were selectively degraded by CPAF when co-incubated in vitro. In addition, specific inhibition T cell antigen presentation by CPAF was correlated with T cell antigen cleavage by CPAF in vitro assay. Conclusions: Our experiments demonstrated that CPAF selectively and specifically degrades chlamydial T cell antigens, which chlamydia may utilize as a novel mechanism for evading host immune responses to promote chlamydia survival.

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Section: Cell-free Degradation Assay and Coomassie Blue Stainingmentioning

confidence: 99%

CPAF selectively degrades chlamydial T cell antigens for inhibiting antigen presentation

Zhang

Zhong

Cai

et al. 2017

J Infect Dev Ctries

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“…28 The common feature distinguishing inclusion proteins, however, is their 50-to 80-amino-acid, bi-lobed, hydrophobic domain that is localized to the inclusion body membrane. 19,23,24,27,29 Currently, at least 9 proteins are identified with this feature, and each inclusion protein has a unique function in the development process of the pathogen. 16,28 Several inclusion proteins have been investigated in terms of function and localization.…”

Section: Inclusion Proteinsmentioning

confidence: 99%

“…24 Second, bioinformatics and modeling suggest that the polar residue located in the center of the motif may organize the coiled coils in the hydrophilic domain into a single amphipathic structure. 27,37 SNAREs have a helix formed with either a glutamine or arginine residue located in the center.…”

Section: Inclusion Protein Amentioning

confidence: 99%

“…2, 4, 5, 7, 9-14, 16, 19-21, 23 The inclusion body has two functions: (1) to protect Chlamydiae during replication and (2) to serve as a gate while the pathogen interacts with its host. 16,24 Using the inclusion, the pathogen successfully eludes endosomes that target foreign matter for degradation by separating from the endocytic pathway early in its development. Chlamydial species are true obligate pathogens because they are unable to synthesize adenosine triphosphate (ATP).…”

Section: Biphasic Development Cyclementioning

confidence: 99%

“…3,23,27 Despite 36 to 59 putative inclusion proteins identified in the C. trachomatis genome, only 23 have been identified between five species (muridarum, cavie, felis, pneumonia, and trachomatis). 23,24 Effector proteins that modify the inclusion body, and are secreted by T3SS, include IncA proteins. IncA from C. trachomatis is the focus of this investigation and described later.…”

Section: Inclusion Proteinsmentioning

confidence: 99%

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Cloning, Expression, and Biophysical Investigations of Truncated Inclusion Protein A (IncA) from Chlamydia trachomatis

Campbell

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ii To my mom and dad, who gave me a thirst for knowledge and the desire to learn.iii Acknowledgements I would like to thank Dr. Linda Columbus for allowing me to work in her lab, study inclusion proteins, and pushing my limits.Thank you Columbus and Mura Lab members for all their technical assistance and feedback.Dr. John D. Shannon for his incredible patience and assistance with MALDI-TOF MS and circular dichroism.Many thanks to Jessica Sarver in the Cafiso lab for allowing me to think out loud about EPR.Thank you to Sandy, Vicki, and Kevin in Facilities Management who kept me laughing, updated me on the news and "goings on" in the department in the "wee" hours of the morning.Special thanks to Tsega Solomon who gave me invaluable technical advice, interesting philosophical debates over lunch, and a renewed interest in shopping. How I will miss you! Special thanks to Dr. Kim Bassett for her listening ear and unconditional friendship. demonstrated the hexa-histidine tag disrupted dimer formation; however, after cleavage of the tag with thrombin, dimer was reformed. Circular dichroism of the construct confirmed the dimer was all α-helical as expected for a SNARE motif. Finally, two single cysteine mutants were prepared and spin-labeled. Continuous wave electron paramagnetic resonance confirmed the sites were spin-labeled and the lineshapes were consistent with moderately immobilized spin labels expected for a tertiary contact. Future double electronelectron resonance experiments will measure the distance between the spin labels, which will elucidate the dimer orientation.

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Pathogenesis of Chlamydia trachomatis in Humans

Guerra

Boga

Rodríguez

et al. 2015

Human Emerging and Re‐emerging Infections

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Characterization of Fifty Putative Inclusion Membrane Proteins Encoded in theChlamydia trachomatisGenome

Cited by 133 publications

References 61 publications

CPAF selectively degrades chlamydial T cell antigens for inhibiting antigen presentation

CPAF selectively degrades chlamydial T cell antigens for inhibiting antigen presentation

Cloning, Expression, and Biophysical Investigations of Truncated Inclusion Protein A (IncA) from Chlamydia trachomatis

Pathogenesis of Chlamydia trachomatis in Humans

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