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针对硫酸化的高分子量小鼠纤毛蛋白的抗体可对毛束和嗅觉黏液层进行染色。

Antibodies to the sulphated, high molecular mass mouse tectorin stain hair bundles and the olfactory mucus layer.

作者信息

Killick R, Richardson G P

机构信息

School of Biological Sciences, University of Sussex, Brighton, UK.

出版信息

Hear Res. 1997 Jan;103(1-2):131-41. doi: 10.1016/s0378-5955(96)00174-8.

Abstract

Polyclonal antibodies were raised in chickens to the glycosylated forms of the high (H), medium (M) and low (L) molecular mass (MM) mouse tectorins. In the mouse cochlea, all three antibodies stained the tectorial membrane. Antibodies raised to HMM tectorin also stained the hair bundles of both inner and outer hair cells. A number of other mouse tissues were screened with the anti-tectorin antibodies to look for similar or antigenically related molecules. Staining was not observed in any other tissue type with the antibodies directed against the MMM and LMM tectorins. In the nose, the anti-HMM tectorin antibodies stained Bowman's glands and the mucus layer overlying the olfactory epithelium. The surface of the adjacent respiratory epithelium was not stained by these antibodies. HMM tectorin can be specifically radiolabelled by injecting neonatal mice with 35SO4 and undergoes a shift in electrophoretic mobility following treatment with keratanase, an endo-beta-galactosidase from Pseudomonas. However, when centrifuged on shallow CsCl gradients HMM tectorin has a buoyant density similar to that of glycoproteins and does not behave as a typical cartilage type proteoglycan. HMM tectorin does not react with mab 5D4, a monoclonal antibody that recognises keratan sulphate glycosaminoglycan from corneal and skeletal muscle proteoglycan. Unlike antibodies to HMM tectorin, mab 5D4 selectively stains the upper surface of the tectorial membrane, Hensen's stripe and the mucus layer overlying the respiratory epithelium. These studies indicate that the MMM and LMM tectorins may be unique to the cochlea, and that HMM may be a "light' keratan sulphate proteoglycan that is antigenically related to either the mucins or a more specific component of the olfactory mucus layer.

摘要

针对高分子量(H)、中分子量(M)和低分子量(L)的糖基化小鼠耳盖蛋白,在鸡体内制备了多克隆抗体。在小鼠耳蜗中,所有三种抗体均能对盖膜进行染色。针对HMM耳盖蛋白产生的抗体也能对内毛细胞和外毛细胞的毛束进行染色。用抗耳盖蛋白抗体对其他一些小鼠组织进行筛选,以寻找相似或抗原相关分子。针对MMM和LMM耳盖蛋白的抗体在任何其他组织类型中均未观察到染色现象。在鼻子中,抗HMM耳盖蛋白抗体对鲍曼腺和覆盖嗅觉上皮的黏液层进行了染色。相邻呼吸上皮的表面未被这些抗体染色。通过给新生小鼠注射35SO4,HMM耳盖蛋白可被特异性放射性标记,在用来自假单胞菌的内切β-半乳糖苷酶角蛋白酶处理后,其电泳迁移率发生改变。然而,当在浅CsCl梯度上离心时,HMM耳盖蛋白的浮力密度与糖蛋白相似,并不表现为典型的软骨型蛋白聚糖。HMM耳盖蛋白不与单克隆抗体mab 5D4反应,mab 5D4可识别来自角膜和骨骼肌蛋白聚糖的硫酸角质素糖胺聚糖。与抗HMM耳盖蛋白的抗体不同,mab 5D4选择性地对盖膜的上表面、亨森带和覆盖呼吸上皮的黏液层进行染色。这些研究表明,MMM和LMM耳盖蛋白可能是耳蜗特有的,而HMM可能是一种“轻度”硫酸角质素蛋白聚糖,在抗原上与黏蛋白或嗅觉黏液层的更特异性成分相关。

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