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Deletion of UDP-glucose pyrophosphorylase reveals a UDP-glucose independent UDP-galactose salvage pathway in Leishmania major

机译:删除UDP-葡萄糖焦磷酸化酶揭示了利什曼原虫主要的UDP-葡萄糖独立的UDP-半乳糖挽救途径

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摘要

The nucleotide sugar UDP-galactose (UDP-Gal) is essential for the biosynthesis of several abundant glycoconjugates forming the surface glycocalyx of the protozoan parasite Leishmania major. Current data suggest that UDP-Gal could arise de novo by epimerization of UDP-glucose (UDP-Glc) or by a salvage pathway involving phosphorylation of Gal and the action of UDP-glucose:α-d-galactose-1-phosphate uridylyltransferase as described by Leloir. Since both pathways require UDP-Glc, inactivation of the UDP-glucose pyrophosphorylase (UGP) catalyzing activation of glucose-1 phosphate to UDP-Glc was expected to deprive parasites of UDP-Gal required for Leishmania glycocalyx formation. Targeted deletion of the gene encoding UGP, however, only partially affected the synthesis of the Gal-rich phosphoglycans. Moreover, no alteration in the abundant Gal-containing glycoinositolphospholipids was found in the deletion mutant. Consistent with these findings, the virulence of the UGP-deficient mutant was only modestly affected. These data suggest that Leishmania elaborates a UDP-Glc independent salvage pathway for UDP-Gal biosynthesis.
机译:核苷酸糖UDP-半乳糖(UDP-Gal)对于生物合成构成原生动物寄生虫利什曼原虫主要表面糖萼的几种丰富的糖结合物至关重要。当前数据表明,UDP-Gal可能通过UDP-葡萄糖(UDP-Glc)的差向异构化或通过涉及Gal磷酸化的补救途径和UDP-葡萄糖的作用而产生:α-d-半乳糖-1-磷酸尿嘧啶转移酶Leloir描述。由于两种途径都需要UDP-Glc,催化UDP-1的葡萄糖-1磷酸活化为UDP-Glc的UDP-葡萄糖焦磷酸化酶(UGP)的失活预计会剥夺利什曼原虫糖萼形成所需的UDP-Gal寄生虫。然而,靶向缺失编码UGP的基因仅部分影响富含Gal的磷酸聚糖的合成。此外,在缺失突变体中未发现丰富的含Gal的糖基肌醇磷脂的改变。与这些发现一致,UGP缺陷型突变体的毒力仅受到中等程度的影响。这些数据表明利什曼原虫详细说明了UDP-Gal生物合成的UDP-Glc独立挽救途径。

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