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利用一种采用聚酯蜡的改良免疫细胞化学方法对大鼠睾丸中的分泌蛋白、膜相关蛋白和细胞骨架蛋白进行定位。

Localization of secretory, membrane-associated and cytoskeletal proteins in rat testis using an improved immunocytochemical protocol that employs polyester wax.

作者信息

Oke B O, Suarez-Quian C A

机构信息

Department of Anatomy and Cell Biology, Georgetown University Medical Center, Washington, District of Columbia 20007.

出版信息

Biol Reprod. 1993 Mar;48(3):621-31. doi: 10.1095/biolreprod48.3.621.

Abstract

Immunocytochemistry is a compromise between maintaining antigenicity and preserving tissue morphology. In the testis, successful immunostaining results at the level of resolution provided by the light microscope have been obtained through use of either frozen or paraffin sections, although both techniques are fraught with limitations. With freezing, tissue preservation is not optimum, whereas with paraffin embedding, antigenicity is often destroyed. These limitations are not trivial and have led to numerous ambiguous results in the literature. In the present study we wish to report the results of immunocytochemical localization of various proteins in testis fixed by perfusion with Bouin's fluid and embedded in polyester wax, a ribboning embedding medium for histology. The advantages of this medium are that it does not require clearing of tissues in xylene solvents before embedding and that unlike paraffin, it liquifies at 38 degrees C. Because of these two properties, the polyester was appears to adequately maintain antigenicity as compared to that observed in frozen sections, yet because it is a ribboning wax, it preserves detailed structure as well as paraffin does. Proteins that were immunolocalized included cytoskeletal proteins (tubulin, actin, vinculin, vimentin) and cell-specific markers: 1) androgen-binding protein (ABP) for Sertoli cells; 2) peripheral type benzodiazepine receptor (PBR) for Leydig cells; and 3) nuclear lamins for germ cells. Biotin-streptavidin peroxidase immunocytochemistry was employed to determine the specific distribution of the various proteins, and both rabbit antisera and mouse monoclonal antibodies were used with equal success. In addition, fluorochrome-labeled second antibodies combined with confocal microscopy were used to examine the disposition of the antigens in the testis. Results revealed maintenance of antigenicity and morphology far superior to that obtained with paraffin and frozen sections, respectively, they also showed that within the seminiferous epithelium, germ cell or Sertoli cell-specific proteins were unambiguously immunolocalized to their respective cells. Specific observations made possible through use of this protocol suggest that neither tubulin or vimentin immunostaining patterns in Sertoli cells are altered during the cycle of the seminiferous epithelium. Similarly, ABP staining appeared constant throughout the cycle. Further, we wish to report that anti-PBR is a specific probe for Leydig cells in vivo and that an anti-nuclear lamin antibody appears to serve as a specific probe for spermatogonia and pachytene spermatocytes, but that the commercially available anti-smooth muscle alpha-actin monoclonal antibody immunostains both the myoid and lymphatic endothelial cells forming the peritubular cells layer of the seminiferous tubule.(ABSTRACT TRUNCATED AT 400 WORDS)

摘要

免疫细胞化学是在保持抗原性和保存组织形态之间的一种折衷方法。在睾丸中,通过使用冷冻切片或石蜡切片,在光学显微镜提供的分辨率水平上已获得成功的免疫染色结果,尽管这两种技术都存在局限性。冷冻时,组织保存并非最佳状态;而石蜡包埋时,抗原性常常被破坏。这些局限性并非微不足道,已导致文献中出现众多模糊的结果。在本研究中,我们希望报告用布安氏液灌注固定并包埋于聚酯蜡(一种用于组织学的带状包埋介质)中的睾丸中各种蛋白质的免疫细胞化学定位结果。这种介质的优点是在包埋前不需要在二甲苯溶剂中清除组织,并且与石蜡不同,它在38摄氏度时会液化。由于这两个特性,与冷冻切片相比,聚酯蜡似乎能充分保持抗原性,但由于它是一种带状蜡,它能像石蜡一样保存详细的结构。进行免疫定位的蛋白质包括细胞骨架蛋白(微管蛋白、肌动蛋白、纽蛋白、波形蛋白)和细胞特异性标志物:1)支持细胞的雄激素结合蛋白(ABP);2)睾丸间质细胞的外周型苯二氮䓬受体(PBR);3)生殖细胞的核纤层蛋白。采用生物素 - 链霉亲和素过氧化物酶免疫细胞化学来确定各种蛋白质的特异性分布,兔抗血清和小鼠单克隆抗体使用效果相同。此外,结合共聚焦显微镜的荧光素标记二抗用于检查睾丸中抗原的分布情况。结果显示,抗原性和形态的保持分别远优于石蜡切片和冷冻切片,它们还表明,在生精上皮内,生殖细胞或支持细胞特异性蛋白质能明确地免疫定位到各自的细胞中。通过使用该方案得以进行的具体观察表明,在生精上皮周期中,支持细胞中的微管蛋白或波形蛋白免疫染色模式均未改变。同样,ABP染色在整个周期中似乎保持恒定。此外,我们希望报告抗PBR是体内睾丸间质细胞的特异性探针,抗核纤层蛋白抗体似乎是精原细胞和粗线期精母细胞的特异性探针,但市售的抗平滑肌α - 肌动蛋白单克隆抗体对形成生精小管周细胞层的肌样细胞和淋巴管内皮细胞均进行免疫染色。(摘要截于400字)

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