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MUC5B中钙依赖性蛋白相互作用在唾液黏液中提供可逆交联。

Calcium-dependent protein interactions in MUC5B provide reversible cross-links in salivary mucus.

作者信息

Raynal Bertrand D E, Hardingham Timothy E, Sheehan John K, Thornton David J

机构信息

Wellcome Trust Centre for Cell-Matrix Research, School of Biological Sciences, 2.205 Stopford Bldg., University of Manchester, Manchester M13 9PT, United Kingdom.

出版信息

J Biol Chem. 2003 Aug 1;278(31):28703-10. doi: 10.1074/jbc.M304632200. Epub 2003 May 19.

Abstract

The macromolecular organization within saliva was investigated by tracer diffusion measurements of fluorescent polystyrene microspheres by fluorescence recovery after photobleaching using a confocal microscope (confocal-FRAP). There was a concentration-dependent reduction in microsphere diffusion; this was much greater in the presence of calcium (10 mm) and was reduced by the addition of EGTA (10 mm). These effects on tracer diffusion showed that native saliva contained a macromolecular organization that was sensitive to free calcium concentrations. This was supported by a major increase in the weight average molecular weight of the high molecular weight mucin fraction in saliva (10-62 x 106) and an increase in intrinsic viscosity of saliva (733 to 1203 ml/g) both caused by calcium. Analysis of the change in tracer diffusion in saliva showed a 20-fold increase in the apparent pore size (from 130 nm in 10 mm CaCl2 to 2600 nm in 10 mm EGTA at physiological concentration). The effect was specific for calcium and was unaffected by up to 2 m NaCl. The calcium binding activity was contained in a high buoyant density fraction of saliva excluded from Sepharose CL-2B. Calcium binding to this fraction gave an approximate Kd of 7 x 10-6 m, and the binding was irreversibly destroyed by treatment with 6 m guanidinium chloride and by mild reduction, suggesting it to be to a protein site. This fraction of saliva was shown to contain MUC5B as the single major protein species by positive ion electrospray ionization-tandem mass spectrometry analysis. The results suggested that oligomeric MUC5B in saliva is assembled into much larger linear or branched assemblies through calcium-mediated protein cross-links.

摘要

通过共聚焦显微镜(共聚焦荧光恢复光漂白法,confocal-FRAP)对荧光聚苯乙烯微球进行示踪扩散测量,研究了唾液中的大分子组织。微球扩散存在浓度依赖性降低;在钙(10 mM)存在的情况下这种降低更为显著,而添加乙二醇双四乙酸(EGTA,10 mM)后则降低。这些对示踪扩散的影响表明,天然唾液含有对游离钙浓度敏感的大分子组织。这一点得到了支持,钙导致唾液中高分子量粘蛋白部分的重均分子量大幅增加(从10-62×106)以及唾液特性粘度增加(从733至1203 ml/g)。对唾液中示踪扩散变化的分析表明,表观孔径增加了20倍(在生理浓度下,从10 mM氯化钙中的130 nm增加到10 mM EGTA中的2600 nm)。这种效应是钙特异性的,高达2 M氯化钠对其无影响。钙结合活性存在于唾液的一个高浮力密度部分中,该部分被琼脂糖CL-2B排除。钙与该部分的结合给出了约7×10-6 M的解离常数(Kd),并且通过用6 M氯化胍处理和轻度还原,这种结合被不可逆地破坏,表明它作用于一个蛋白质位点。通过正离子电喷雾电离串联质谱分析表明,该唾液部分含有MUC5B作为单一主要蛋白质种类。结果表明,唾液中的寡聚MUC5B通过钙介导的蛋白质交联组装成更大的线性或分支聚集体。

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