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大鼠海曼肾炎免疫电子显微镜研究中的固定和包埋变量

Fixation and embedding variables in the immuno-electron microscopic study of rat Heymann nephritis.

作者信息

Rantala I, Helin H, Helin M, Kotti V, Pasternack A

出版信息

Histochemistry. 1980;66(2):189-99. doi: 10.1007/BF00494645.

Abstract

Fixation and embedding variables were compared in immuno-electron microscopic localization of rat IgG in an autologous immune complex-type nephritis. Specimens from kidney cortex were fixed for 3, 6 or 9 h in the following fixatives made in 0.1 M phosphate buffer at pH 7.4: 4% paraformaldehyde, 2.5% glutaraldehyde, periodate- lysine-paraformaldehyde or modified Karnovsky's fixative. Localization of IgG was performed on tissue sections cut with a tissue chopper, cryostat or sliding microtome, using agarose, Ames O.C.T. Compound or polyethylene glycol respectively as cutting matrixes. The sections were incubated in peroxidase-labelled antirat IgG antiserum (diluted 1:20 with phosphate-buffered saline) for 60 h. Peroxidase activity was then revealed and the sections embedded in Epon. Exact localization of IgG throughout the sections and good ultrastructure were achieved when paraformaldehyde and agarose were used. Periodatelysine-paraformaldehyde proved almost as useful as paraformaldehyde in connection with agarose in respect of peroxidase reaction and ultrastructure. Fixatives containing glutaraldehyde gave a mostly weak and unevenly distributed peroxidase reaction product. In the cryostat sections breaking of the tissue structure could not be avoided. When polyethylene glycol was used as cutting matrix no peroxidase reaction was achieved.

摘要

在自体免疫复合型肾炎大鼠IgG的免疫电子显微镜定位研究中,对固定和包埋变量进行了比较。取肾皮质标本,在pH 7.4的0.1 M磷酸盐缓冲液中配制的下列固定剂中分别固定3、6或9小时:4%多聚甲醛、2.5%戊二醛、高碘酸盐-赖氨酸-多聚甲醛或改良的卡诺夫斯基固定剂。使用组织切片机、低温恒温切片机或滑动切片机切割组织切片,分别以琼脂糖、Ames O.C.T. 复合物或聚乙二醇作为切割基质,进行IgG的定位。将切片在过氧化物酶标记的抗大鼠IgG抗血清(用磷酸盐缓冲盐水稀释1:20)中孵育60小时。然后显示过氧化物酶活性,并将切片包埋在环氧树脂中。当使用多聚甲醛和琼脂糖时,可在整个切片中实现IgG的精确定位并获得良好的超微结构。就过氧化物酶反应和超微结构而言,高碘酸盐-赖氨酸-多聚甲醛与多聚甲醛加琼脂糖几乎同样有效。含戊二醛的固定剂产生的过氧化物酶反应产物大多较弱且分布不均。在低温恒温切片中,组织结构的破坏无法避免。当使用聚乙二醇作为切割基质时,未获得过氧化物酶反应。

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