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一种来自偶发分枝杆菌的新型含丝氨酸糖肽脂。

A new type of serine-containing glycopeptidolipid from Mycobacterium xenopi.

作者信息

Rivière M, Puzo G

机构信息

Centre de Recherche de Biochimie et Génétique Cellulaires, Centre National de la Recherche Scientifique, Toulouse, France.

出版信息

J Biol Chem. 1991 May 15;266(14):9057-63.

PMID:1902834
Abstract

An unknown immunogenic glycopeptidolipid, named GPL X-1, was isolated from Mycobacterium xenopi, which is a nontuberculous mycobacterium responsible for pulmonary and disseminated infectious diseases mainly occurring in immunocompromised patients. The glycopeptidolipid was purified until homogeneity, in the native form, by direct phase high performance liquid chromatography. A new route is proposed for the structural elucidation of its unusual lipopeptidic core. The presence of allothreonine (aThr), phenylalanine, and serine in the molecular ratio 1:1:2, respectively, was established by reverse phase high performance liquid chromatography analysis of the phenylthiocarbamyl amino acid derivatives. From the molecular mass (1828 Da) of the native glycopeptidolipid, determined by cesium ion liquid secondary ion mass spectrometry using the amphipathic triethylene glycol monobutyl ether matrix, it was deduced that the tetrapeptide was amidified by a dodecanoic acid. The complete structure, C12-Ser-Ser-Phe-aThr-OCH3, of the lipopeptidic core was established by pyrolysis electron impact-mass spectrometry of the native glycopeptidolipid. To date, this is the first example of a mycobacterial glycopeptidolipid with a C12-tetrapeptidic core containing serine. A novel approach, based on two dimensional 1H,1H correlated spectroscopy analysis of the native and peracetylated GPL X-1, was developed, allowing the structural determination of the monosaccharidic residues with their alkali-labile groups "in situ" on the whole complex molecule. 2-O-Acyl-alpha-L-Rhap, alpha-L-Rhap, 2,4-di-O-acyl-6-deoxy-alpha-L-Glcp, 2,3,4-tri-O-Me-alpha-L-Rhap, and 3-O-Me-6-deoxy-alpha-L-Talp were identified, where Me, Rhap, and Talp are methyl, rhamnopyranosyl, and talopyranosyl, respectively. The latter two were localized at the carbohydrate non-reducing ends, and the C-3's of the remaining monosaccharide residues were found involved in the interglycosidic linkage. The alpha anomeric configurations were inferred from the JC-1,H-1 heteronuclear coupling constants, and the L absolute configurations for all the monosaccharide residues were established by gas chromatography analysis of the trimethylsilyl (+/-)-2-butyl glycosides. Finally, by pyrolysis electron impact mass spectrometry of peracetylated GPL X-1, the following tetrasaccharide appendage structure was proposed: 2,3,4-tri-O-Me-L-Rhap(alpha 1----3)-2-O-lauryl-L-Rhap(alpha 1----3)-L-Rhap- (alpha 1----3)-2,4-di-O-(acetyl,lauryl)-6-deoxy-alpha-L-Glcp. Compared to the oligosaccharidic glycopeptidolipid structures, the particular features of the GPL X-1 tetrasaccharide structure arise from the presence of monosaccharide residues esterified by C12 fatty acids and from the absence of the basal disaccharide core, L-Rhap-(alpha 1----2)-6-deoxy-alpha-L-Talp.(ABSTRACT TRUNCATED AT 400 WORDS)

摘要

从蟾分枝杆菌中分离出一种未知的免疫原性糖肽脂,命名为GPL X-1。蟾分枝杆菌是一种非结核分枝杆菌,主要引起免疫功能低下患者的肺部感染和播散性感染疾病。通过直接相高效液相色谱法将该糖肽脂纯化至均一的天然形式。提出了一种新的方法来阐明其不同寻常的脂肽核心结构。通过对苯硫代氨基甲酰氨基酸衍生物进行反相高效液相色谱分析,确定了别苏氨酸(aThr)、苯丙氨酸和丝氨酸的分子比例分别为1:1:2。使用两亲性三甘醇单丁醚基质通过铯离子液体二次离子质谱法测定天然糖肽脂的分子量(1828 Da),由此推断四肽被十二烷酸酰胺化。通过对天然糖肽脂进行热解电子轰击质谱分析,确定了脂肽核心的完整结构为C12-Ser-Ser-Phe-aThr-OCH3。迄今为止,这是首个具有含丝氨酸的C12-四肽核心的分枝杆菌糖肽脂实例。开发了一种基于对天然和全乙酰化GPL X-1进行二维1H,1H相关光谱分析的新方法,能够在整个复合分子上“原位”确定单糖残基及其碱不稳定基团的结构。鉴定出了2-O-酰基-α-L-鼠李糖、α-L-鼠李糖、2,4-二-O-酰基-6-脱氧-α-L-葡萄糖、2,3,4-三-O-甲基-α-L-鼠李糖和3-O-甲基-6-脱氧-α-L-塔罗糖,其中Me、Rhap和Talp分别代表甲基、鼠李吡喃糖基和塔罗吡喃糖基。后两者位于碳水化合物的非还原端,其余单糖残基的C-3参与糖苷键连接。从JC-1,H-1异核耦合常数推断出α异头构型,通过对三甲基硅烷基(±)-2-丁基糖苷进行气相色谱分析确定了所有单糖残基的L绝对构型。最后,通过对全乙酰化GPL X-1进行热解电子轰击质谱分析,提出了以下四糖附属结构:2,3,4-三-O-甲基-L-鼠李糖(α1→3)-2-O-月桂酰-L-鼠李糖(α1→3)-L-鼠李糖-(α1→3)-2,4-二-O-(乙酰基,月桂酰)-6-脱氧-α-L-葡萄糖。与寡糖糖肽脂结构相比,GPL X-1四糖结构的独特特征源于存在被C12脂肪酸酯化的单糖残基以及不存在基础二糖核心L-鼠李糖-(α1→2)-6-脱氧-α-L-塔罗糖。(摘要截选至400字)

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