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系统性的胶囊基因破坏揭示了半乳糖代谢在新型隐球菌毒力中的核心作用。

Systematic capsule gene disruption reveals the central role of galactose metabolism on Cryptococcus neoformans virulence.

作者信息

Moyrand Frédérique, Fontaine Thierry, Janbon Guilhem

机构信息

Unité de Mycologie Moléculaire, CNRS URA3012, Institut Pasteur, France.

出版信息

Mol Microbiol. 2007 May;64(3):771-81. doi: 10.1111/j.1365-2958.2007.05695.x.

Abstract

The polysaccharidic capsule is the main virulence factor of Cryptococcus neoformans. It primarily comprised of two polysaccharides: glucuronoxylomannan (GXM, 88% of the capsule mass) and galactoxylomannan (GalXM, 7% of the capsule mass). We constructed a large collection of mutant strains in which genes potentially involved in capsule biosynthesis were deleted. We used a new post-genomic approach to study the virulence of the strains. Primers specific for unique tags associated with the disruption cassette were used in a real-time PCR virulence assay to measure the fungal burden of each strain in different organs of mice in multi-infection experiments. With this very sensitive assay, we identified a putative UDP-glucose epimerase (Uge1p) and a putative UDP-galactose transporter (Ugt1p) essential for C. neoformans virulence. The uge1Delta and ugt1Delta strains are temperature sensitive and do not produce GalXM but synthesize a larger capsule. These mutant strains (GalXM negative, GXM positive) are not able to colonize the brain even at the first day of infection whereas GXM-negative strains (GalXM positive) can still colonize the brain, although less efficiently than the wild-type strain.

摘要

多糖荚膜是新型隐球菌的主要毒力因子。它主要由两种多糖组成:葡糖醛酸木甘露聚糖(GXM,占荚膜质量的88%)和半乳糖木甘露聚糖(GalXM,占荚膜质量的7%)。我们构建了大量突变菌株,其中潜在参与荚膜生物合成的基因被删除。我们采用一种新的后基因组方法来研究这些菌株的毒力。在多重感染实验中,用于与破坏盒相关的独特标签的特异性引物被用于实时PCR毒力测定,以测量每种菌株在小鼠不同器官中的真菌负荷。通过这种非常灵敏的测定方法,我们鉴定出一种推定的UDP-葡萄糖表异构酶(Uge1p)和一种推定的UDP-半乳糖转运蛋白(Ugt1p),它们对新型隐球菌的毒力至关重要。uge1Δ和ugt1Δ菌株对温度敏感,不产生GalXM,但合成更大的荚膜。这些突变菌株(GalXM阴性,GXM阳性)即使在感染的第一天也无法在脑部定殖,而GXM阴性菌株(GalXM阳性)仍然可以在脑部定殖,尽管效率低于野生型菌株。

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