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克氏锥虫蝶啶还原酶2与底物及抑制剂复合物的晶体结构

Crystal structure of Trypanosoma cruzi pteridine reductase 2 in complex with a substrate and an inhibitor.

作者信息

Schormann Norbert, Pal Biswajit, Senkovich Olga, Carson Mike, Howard Andrew, Smith Craig, Delucas Lawrence, Chattopadhyay Debasish

机构信息

Center for Biophysical Sciences and Engineering, University of Alabama at Birmingham, Birmingham, AL 35294, USA.

出版信息

J Struct Biol. 2005 Oct;152(1):64-75. doi: 10.1016/j.jsb.2005.07.008.

Abstract

Reduced pteridines are required for a number of important cellular functions. Trypanosomatid parasites, unlike their mammalian hosts, are pteridine auxotrophs and salvage the precursor pteridines from the host and reduce them to the respective biologically active tetrahydro forms using parasite-encoded enzymes. These enzymes may offer selective drug targets. In Leishmania, pteridine reductase 1 (PTR1), the primary enzyme for reducing pterins, is also responsible for resistance to antifolate drugs. Typically, PTR1 is more active with fully oxidized biopterin and folate than with their reduced counterparts. We have identified an enzyme, TcPTR2 of Trypanosoma cruzi, which though very similar to PTR1 in its primary sequence, can reduce only dihydrobiopterin and dihydrofolate and not oxidized pteridines. The structures of an inhibitor (methotrexate) and a substrate (dihydrofolate) complex of this enzyme demonstrate that the orientation of the substrate and the inhibitor in the active site of TcPTR2 are different from each other. However, the orientation of each ligand is similar to that of the corresponding ligand in Leishmania major PTR1 complexes.

摘要

多种重要的细胞功能都需要还原型蝶啶。与它们的哺乳动物宿主不同,锥虫类寄生虫是蝶啶营养缺陷型,它们从宿主中获取蝶啶前体,并利用寄生虫编码的酶将其还原为各自具有生物活性的四氢形式。这些酶可能成为选择性药物靶点。在利什曼原虫中,蝶啶还原酶1(PTR1)是还原蝶呤的主要酶,它也与抗叶酸药物耐药性有关。通常,PTR1对完全氧化的生物蝶呤和叶酸的活性比对其还原形式的活性更高。我们鉴定出一种酶,即克氏锥虫的TcPTR2,它虽然在一级序列上与PTR1非常相似,但只能还原二氢生物蝶呤和二氢叶酸,而不能还原氧化型蝶啶。这种酶的一种抑制剂(甲氨蝶呤)和一种底物(二氢叶酸)复合物的结构表明,底物和抑制剂在TcPTR2活性位点中的取向彼此不同。然而,每种配体的取向与大利什曼原虫PTR1复合物中相应配体的取向相似。

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