cPLA2 Regulates the Expression of Type I Interferons and Intracellular Immunity to Chlamydia trachomatis

Background: C. trachomatis has a reduced genome and was thought to obtain phospholipids as well as other nutrients from the host. Results:The new phospholipid molecular species that appear in infected cells are produced by C. trachomatis. Conclusion: C. trachomatis needs only glucose, isoleucine, and serine to synthesize its own membrane phospholipids. Significance: C. trachomatis relies on autonomous phospholipid synthesis.

Section: Discussionsupporting

confidence: 71%

Section: Phospholipid Content and Synthesis In Ctr-infected Helamentioning

confidence: 70%

Chlamydia trachomatis Relies on Autonomous Phospholipid Synthesis for Membrane Biogenesis

Yao

Cherian

Frank

et al. 2015

“…This work was also supported by the American Lebanese Syrian Associated Charities. The atomic coordinates and structure factors (code 4Q9N) cells found that a decrease in cPLA 2 activity has no effect on C. trachomatis growth (5). In mouse cells, cPLA 2 knockdown increases chlamydial titers, suggesting that cPLA 2 is more likely involved in intracellular immunity (5).…”

mentioning

confidence: 99%

“…The atomic coordinates and structure factors (code 4Q9N) cells found that a decrease in cPLA 2 activity has no effect on C. trachomatis growth (5). In mouse cells, cPLA 2 knockdown increases chlamydial titers, suggesting that cPLA 2 is more likely involved in intracellular immunity (5). One function of FASII is to generate the 3-hydroxy fatty acids for lipopolysaccharide synthesis in Gram-negative bacteria (6).…”

mentioning

confidence: 99%

Type II Fatty Acid Synthesis Is Essential for the Replication of Chlamydia trachomatis

Yao

AbdelRahman

Robertson

et al. 2014

Background: Chlamydia trachomatis has a phospholipid composition that resembles its eukaryotic host, but it contains branched-chain fatty acids of chlamydial origin. Results: The inhibition of the enoyl-acyl carrier protein reductase (FabI) in chlamydial fatty acid synthesis blocks C. trachomatis replication. Conclusion: Bacterial FASII is required for C. trachomatis proliferation. Significance: FabI is a therapeutic target against C. trachomatis.

“…Previous work from our laboratory and others has demonstrated that the IRGM (GMS) proteins play a particularly important role in innate immune resistance to intracellular bacteria and protozoa in mice (8, 14, 16 -26). Absence of Irgm1, for instance, leads to a striking susceptibility to multiple organisms, including Toxoplasma gondii (8,19), Salmonella typhimurium (25), Listeria monocytogenes (19), Chlamydia trachomatis (27,28), and Mycobacterium species (20, 21). In comparison, absence of the GKS proteins Irgd or Irga6 results in relatively weak phenotypes (8,13,19).…”

mentioning

confidence: 99%

Immunity-related GTPase M (IRGM) Proteins Influence the Localization of Guanylate-binding Protein 2 (GBP2) by Modulating Macroautophagy

Traver

Henry

Cantillana

et al. 2011

Self Cite

The immunity-related GTPases (IRGs) are a family of proteins induced by interferon-␥ that play a crucial role in innate resistance to intracellular pathogens. The M subfamily of IRG proteins (IRGM) plays a profound role in this context, in part because of the ability of its members to regulate the localization and expression of other IRG proteins. We present here evidence that IRGM proteins affect the localization of the guanylatebinding proteins (GBPs), a second family of interferon-induced GTP-binding proteins that also function in innate immunity. Absence of Irgm1 or Irgm3 led to accumulation of Gbp2 in intracellular compartments that were positive for both the macroautophagy (hereafter referred to as autophagy) marker LC3 and the autophagic adapter molecule p62/Sqstm1. Gbp2 was similarly relocalized in cells in which autophagy was impaired because of the absence of Atg5. Both in Atg5-and IRGM-deficient cells, the IRG protein Irga6 relocalized to the same compartments as Gbp2, raising the possibility of a common regulatory mechanism. However, other data indicated that Irga6, but not Gbp2, was ubiquitinated in IRGM-deficient cells. Similarly, coimmunoprecipitation studies indicated that although Irgm3 did interact directly with Irgb6, it did not interact with Gbp2. Collectively, these data suggest that IRGM proteins indirectly modulate the localization of GBPs through a distinct mechanism from that through which they regulate IRG protein localization. Further, these results suggest that a core function of IRGM proteins is to regulate autophagic flux, which influences the localization of GBPs and possibly other factors that instruct cell-autonomous immune resistance.The innate immune system is comprised of multiple effector pathways that are induced in host cells by proinflammatory cytokines such as IFN-␥. Such effectors confer on the host cells the ability to more easily eradicate invading pathogens through diverse mechanisms (1-4). A prominent family of IFN-␥-induced proteins that are required for resistance to intracellular bacteria and protozoa are the immunity-related GTPases. IRG 2 proteins share a number of biochemical functions: they are GTPases (5, 6), they bind lipid membranes in various intracellular membrane compartments (6 -8), and they form dimers and/or oligomers (5, 9). These and other characteristics relate them to the dynamins, a large family of GTPbinding proteins that are involved in vesicle formation, vesicle trafficking, and other aspects of lipid membrane remodeling (10 -12). Like the dynamins, current models suggest that the IRGs modulate membrane processing in cells (8, 13), which in turn impacts pathogen survival and/or leukocyte functioning.IRG proteins can be separated into the IRGA, IRGB, IRGC, IRGD, and IRGM subfamilies based on homology across the GTP-binding domain (14). Proteins in the IRGM subfamily are distinguished from the other proteins by possessing a non-canonical GMS sequence in the first GTP-binding motif (G1), whereas the remaining subfamilies all possess the canonical...