首页> 美国卫生研究院文献>Biochemical Journal >Physical characterization of a low-charge glycoform of the MUC5B mucin comprising the gel-phase of an asthmatic respiratory mucous plug.
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Physical characterization of a low-charge glycoform of the MUC5B mucin comprising the gel-phase of an asthmatic respiratory mucous plug.

机译:MUC5B粘蛋白的低电荷糖型的物理特征包括哮喘呼吸道粘液栓的凝胶相。

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摘要

We have previously noted that sequential extraction of an asthmatic mucous exudate with 6 M guanidinium chloride yielded a fraction of the mucins that were most resistant to solubilization and of high Mr [Sheehan, Richardson, Fung, Howard and Thornton (1995) Am. J. Respir. Cell Mol. Biol. 13, 748-756]. Here we show that this mucin fraction is dominated (at least 96% of the total) by the low-charge glycoform of the MUC5B gene product. Seen in the electron microscope the mucins appeared mainly as compact 'island' structures composed of linear threads often emanating from globular 'nodes' rather than the discrete linear threads more typical of mucins that we have previously described. The effect of reducing agents was as expected for other gel-forming mucins, i.e. reduced subunits or monomers of Mr 3x10(6)) were produced within 15 min of treatment. Kinetic experiments on the cleavage of the intact mucins with the proteinase trypsin indicated two clear regimes of fragmentation. An initial rapid cleavage generated mucins ranging from Mr=4x10(6) to 30x10(6) that in the electron microscope appeared as polydisperse threads (500-3000 nm in length), similar to normal and other respiratory mucins that we have previously characterized. A subsequent slower fragmentation over many hours yielded a major fragment of Mr 3x10(6) and length 200-600 nm, very similar in size and Mr to the subunits obtained by reduction. The results suggest that the MUC5B mucin is assembled, first into polydisperse linear threads, which are then linked together via a protein-mediated process. This might involve part of the mucin polypeptide or an as yet unidentified protein(s). The high proteinase susceptibility of the linkage suggests that it might be a point of control for mucin size and thus mucus rheology.
机译:我们以前曾指出,用6 M氯化胍顺序提取哮喘粘液渗出液产生的部分黏蛋白对增溶性的抵抗力最高,并且具有很高的黏附度[Sheehan,Richardson,Fung,Howard和Thornton(1995)Am。 J.呼吸。细胞分子生物学13,748-756]。在这里,我们显示该粘蛋白部分被MUC5B基因产物的低电荷糖型所主导(至少占总数的96%)。在电子显微镜下看到的粘蛋白主要表现为紧凑的“岛状”结构,该结构通常由球形“节点”发出,而不是我们先前描述的粘蛋白中更典型的离散线性线。还原剂的作用与其他形成凝胶的粘蛋白一样,即在处理的15分钟内产生了还原的亚基或Mr 3x10(6)的单体。用蛋白酶胰蛋白酶切割完整粘蛋白的动力学实验表明有两种清晰的片段化方案。最初的快速裂解产生的粘蛋白范围从Mr = 4x10(6)到30x10(6),在电子显微镜下显示为多分散线(长度为500-3000 nm),类似于我们先前表征的正常和其他呼吸道粘蛋白。随后在许多小时内较慢的碎裂产生了3x10(6)先生的主要片段,长度为200-600 nm,其大小和Mr与通过还原获得的亚基非常相似。结果表明,MUC5B粘蛋白首先组装成多分散线性线,然后通过蛋白质介导的过程连接在一起。这可能涉及粘蛋白多肽的一部分或尚未鉴定的蛋白质。连接的高蛋白酶敏感性表明,它可能是控制粘蛋白大小和粘液流变性的控制点。

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