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青蛙肠系膜微血管内皮细胞表面白蛋白的免疫过氧化物酶标记。

Immunoperoxidase labelling of albumin at the endothelial cell surface of frog mesenteric microvessels.

作者信息

Clough G, Moffitt H

机构信息

Department of Physiology and Biophysics, St Mary's Hospital Medical School, London, United Kingdom.

出版信息

Int J Microcirc Clin Exp. 1992 Nov;11(4):345-58.

PMID:1459795
Abstract

Albumin was visualised at the endothelial cell surface of perfused frog mesenteric microvessels using immuno-peroxidase labelling. Vessels in the mesenteries of pithed frogs were washed free of blood and then perfused with frog Ringer solutions containing bovine serum albumin (BSA) at a concentration of 20 mg BSA ml-1, followed by a brief Ringer flush to remove excess albumin from the vessel lumen. The tissues were fixed in 1% glutaraldehyde and a double antibody labelling technique used to identify albumin within the tissue. A dense layer of peroxidase reaction product was seen, which extended 25-50 nm into the vessel lumen. It appeared as a continuous layer lining the luminal openings of interendothelial cell clefts and vesicles open to the luminal cell surface. In some vessels a more irregular layer of peroxidase labelled albumin was seen extending 150 to 200 nm into the vessel lumen, whilst in others clumps of peroxidase labelled albumin were also seen within the vessel lumen. These data offer direct evidence that BSA does interact with the endothelial cell surface of perfused frog mesenteric microvessels but suggest that a proportion is loosley or non-specifically bound to the cell surface and can be removed by a brief Ringer flush. The remainder appears more tightly bound and resistant to Ringer flush.

摘要

采用免疫过氧化物酶标记法,在灌注的蛙肠系膜微血管内皮细胞表面观察到白蛋白。将处死的蛙肠系膜中的血管冲洗去除血液,然后用含有浓度为20 mg BSA/ml牛血清白蛋白(BSA)的蛙林格氏液灌注,随后用林格氏液短暂冲洗以去除血管腔内多余的白蛋白。组织用1%戊二醛固定,并采用双抗体标记技术鉴定组织内的白蛋白。可见一层致密的过氧化物酶反应产物,延伸至血管腔内25 - 50 nm。它表现为一层连续的层,衬在内皮细胞间裂孔和通向管腔细胞表面的小泡的管腔开口处。在一些血管中,可见一层更不规则的过氧化物酶标记的白蛋白延伸至血管腔内150至200 nm,而在其他血管中,在血管腔内也可见过氧化物酶标记的白蛋白团块。这些数据提供了直接证据,表明BSA确实与灌注的蛙肠系膜微血管内皮细胞表面相互作用,但表明一部分以松散或非特异性方式结合在细胞表面,可通过林格氏液短暂冲洗去除。其余部分似乎结合更紧密,对林格氏液冲洗有抗性。

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