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V型胶原蛋白:鸡α1(V)氨基末端结构域的分子结构和纤维组织,角膜纤维生成的假定调节因子。

Type V collagen: molecular structure and fibrillar organization of the chicken alpha 1(V) NH2-terminal domain, a putative regulator of corneal fibrillogenesis.

作者信息

Linsenmayer T F, Gibney E, Igoe F, Gordon M K, Fitch J M, Fessler L I, Birk D E

机构信息

Department of Anatomy and Cellular Biology, Tufts University Medical School, Boston, Massachusetts 02111.

出版信息

J Cell Biol. 1993 Jun;121(5):1181-9. doi: 10.1083/jcb.121.5.1181.

Abstract

Previous work from our laboratories has demonstrated that: (a) the striated collagen fibrils of the corneal stroma are heterotypic structures composed of type V collagen molecules coassembled along with those of type I collagen, (b) the high content of type V collagen within the corneal collagen fibrils is one factor responsible for the small, uniform fibrillar diameter (25 nm) characteristic of this tissue, (c) the completely processed form of type V collagen found within tissues retains a large noncollagenous region, termed the NH2-terminal domain, at the amino end of its alpha 1 chain, and (d) the NH2-terminal domain may contain at least some of the information for the observed regulation of fibril diameters. In the present investigation we have employed polyclonal antibodies against the retained NH2-terminal domain of the alpha 1(V) chain for immunohistochemical studies of embryonic avian corneas and for immunoscreening a chicken cDNA library. When combined with cDNA sequencing and molecular rotary shadowing, these approaches provide information on the molecular structure of the retained NH2-terminal domain as well as how this domain might function in the regulation of fibrillar structure. In immunofluorescence and immunoelectron microscopy analyses, the antibodies against the NH2-terminal domain react with type V molecules present within mature heterotypic fibrils of the corneal stroma. Thus, epitopes within at least a portion of this domain are exposed on the fibril surface. This is in marked contrast to mAbs which we have previously characterized as being directed against epitopes located in the major triple helical domain of the type V molecule. The helical epitopes recognized by these antibodies are antigenically masked on type V molecules that have been assembled into fibrils. Sequencing of the isolated cDNA clones has provided the conceptual amino acid sequence of the entire amino end of the alpha 1(V) procollagen chain. The sequence shows the location of what appear to be potential propeptidase cleavage sites. One of these, if preferentially used during processing of the type V procollagen molecule, can provide an explanation for the retention of the NH2-terminal domain in the completely processed molecule. The sequencing data also suggest that the NH2-terminal domain consists of several regions, providing a structure which fits well with that of the completely processed type V molecule as visualized by rotary shadowing.

摘要

我们实验室之前的研究表明

(a) 角膜基质的横纹状胶原纤维是由 V 型胶原分子与 I 型胶原分子共同组装而成的异型结构;(b) 角膜胶原纤维中 V 型胶原的高含量是导致该组织具有小而均匀的纤维直径(25 纳米)这一特征的因素之一;(c) 在组织中发现的完全加工形式的 V 型胶原在其α1 链的氨基末端保留了一个大的非胶原区域,称为 NH2 末端结构域;(d) NH2 末端结构域可能包含至少一些观察到的纤维直径调节信息。在本研究中,我们使用了针对α1(V)链保留的 NH2 末端结构域的多克隆抗体,对鸡胚角膜进行免疫组织化学研究,并对鸡 cDNA 文库进行免疫筛选。当与 cDNA 测序和分子旋转投影相结合时,这些方法提供了关于保留的 NH2 末端结构域的分子结构以及该结构域在纤维结构调节中可能如何发挥作用的信息。在免疫荧光和免疫电子显微镜分析中,针对 NH2 末端结构域的抗体与角膜基质成熟异型纤维中存在的 V 型分子发生反应。因此,该结构域至少一部分内的表位暴露在纤维表面。这与我们之前鉴定为针对位于 V 型分子主要三螺旋结构域中的表位的单克隆抗体形成鲜明对比。这些抗体识别的螺旋表位在已组装成纤维的 V 型分子上被抗原性掩盖。对分离的 cDNA 克隆进行测序,得到了α1(V)前胶原链整个氨基末端的概念性氨基酸序列。该序列显示了似乎是潜在前肽酶切割位点的位置。如果其中一个位点在 V 型前胶原分子加工过程中被优先使用,那么这可以解释为什么在完全加工的分子中保留了 NH2 末端结构域。测序数据还表明,NH2 末端结构域由几个区域组成,其结构与通过旋转投影观察到的完全加工的 V 型分子的结构非常吻合。

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