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胶原蛋白V前体中的酪氨酸硫酸化

Tyrosine sulfation in precursors of collagen V.

作者信息

Fessler L I, Brosh S, Chapin S, Fessler J H

出版信息

J Biol Chem. 1986 Apr 15;261(11):5034-40.

PMID:3082875
Abstract

Radioactive labeling of p-collagens V, collagens V, and, to a small extent, of procollagen V occurred when [35S]sulfate was incubated with tendons or primary tendon cell cultures, or blood vessels and crops of 17- to 19-day-old chick embryos, or with lung slices from neonatal rats. Most or all of this label is in the form of 1 or more sulfated tyrosine residues/chain of p alpha 1(V), alpha 1(V), p alpha 1'(V), alpha 1'(V), p alpha 2(V), and alpha 2(V), and it remains attached through purification by dialysis, ammonium sulfate precipitation, CsCl-GdnCl2 equilibrium buoyant density and velocity sedimentations, ion-exchange chromatography, and sodium dodecyl sulfate gel electrophoresis. Radioactive tyrosine sulfate was identified in alkaline hydrolysates of these collagen V chains, after labeling the tissues with either [35S]sulfate or [3H]tyrosine, by electrophoretic and chromatographic comigration with a tyrosine sulfate standard. Tunicamycin A1, which inhibits the attachment of N-linked complex carbohydrate, did not interfere with the sulfation process. The tyrosine sulfate is located in a noncollagenous domain, which is probably adjacent to the amino end of the collagen helix, and is retained throughout the physiological proteolytic processing of procollagens V. After digestion with Staphylococcus aureus V8 protease, 35S-labeled p alpha 1(V) and alpha 1(V) chains gave the same map of labeled peptides, and this differed from the map given by p alpha 1'(V) and alpha 1'(V) chains. Little sulfation of p alpha 2(V) and alpha 2(V) chains occurs. The implications of these observations for the structure and properties of procollagens V and their derivatives are considered.

摘要

当将[35S]硫酸盐与肌腱或原代肌腱细胞培养物、17至19日龄鸡胚的血管和嗉囊,或新生大鼠的肺切片一起孵育时,会出现对Ⅴ型原胶原、Ⅴ型胶原以及少量前胶原Ⅴ的放射性标记。这些标记中的大部分或全部以1个或更多个硫酸化酪氨酸残基/ pα1(Ⅴ)、α1(Ⅴ)、pα1'(Ⅴ)、α1'(Ⅴ)、pα2(Ⅴ)和α2(Ⅴ)链的形式存在,并且通过透析、硫酸铵沉淀、CsCl-GdnCl2平衡浮力密度和速度沉降、离子交换色谱法以及十二烷基硫酸钠凝胶电泳进行纯化后,它仍然附着在上面。在用[35S]硫酸盐或[3H]酪氨酸标记组织后,通过与硫酸酪氨酸标准品进行电泳和色谱共迁移,在这些Ⅴ型胶原链的碱性水解产物中鉴定出放射性硫酸酪氨酸。抑制N-连接复合碳水化合物附着的衣霉素A1并不干扰硫酸化过程。硫酸酪氨酸位于一个非胶原结构域中,该结构域可能与胶原螺旋的氨基末端相邻,并且在前胶原Ⅴ的整个生理蛋白水解加工过程中都保留下来。用金黄色葡萄球菌V8蛋白酶消化后,35S标记的pα1(Ⅴ)和α1(Ⅴ)链给出了相同的标记肽图谱,这与pα1'(Ⅴ)和α1'(Ⅴ)链给出的图谱不同。pα2(Ⅴ)和α2(Ⅴ)链几乎没有硫酸化。考虑了这些观察结果对前胶原Ⅴ及其衍生物的结构和性质的影响。

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