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对患有遗传性吸收不良综合征患者的富含脂质肠细胞进行超微结构免疫金标记。

Ultrastructural immunogold labeling of lipid-laden enterocytes from patients with genetic malabsorption syndromes.

作者信息

Samson-Bouma M E, Verthier N, Ginsel L A, Feldmann G, Fransen J A, Aggerbeck L P

机构信息

U327, Institut National de la Santé et de la Recherche Médicale, Faculté de Médecine Xavier Bichat, Université Paris 7-Denis Diderot, France.

出版信息

Biol Cell. 1996;87(3):189-96.

PMID:9075328
Abstract

Intestinal biopsies from patients having genetic disorders of lipoprotein assembly and secretion, such as abetalipoproteinemia (ABL) or Anderson's disease (AD), contain large amounts of lipids which are accumulated in the enterocytes. Determination of the intracellular sites in which the lipids accumulate and to which apolipoproteins the lipids are bound would help to identify the defects in these diseases and further elucidate the mechanisms by which lipoprotein assembly and secretion occur normally. Ultrastructural immunogold labeling, however, is hampered by the poor preservation of the lipids accumulated in the enterocytes of these patients. We have used routine electron microscopy (fixation and ultra-thin sectioning) along with three methods for immunogold labeling of lipid-laden enterocytes: ultrathin cryosectioning, low temperature freeze substitution with embedding in Lowicryl K4M, and ultra-low temperature freeze substitution with embedding in Lowicryl HM20, to establish a protocol for investigating the intestinal tissue from these patients. Ultracryosectioning, while preserving the overall morphology of the lipid laden enterocytes, did not preserve the lipid content and the immunogold labeling of apolipoprotein B (ApoB) appeared dislocated. Freeze substitution and low temperature embedding in Lowicryl K4M, in contrast, appeared to better preserve the lipid and lipoprotein structures; however, the antigenicity of both apoAI and apoB appeared to be lost and no specific labeling could be obtained. Freeze substitution and embedding in Lowicryl HM20 best preserved the lipid and lipoprotein structures while maintaining apoprotein antigenicity. In conclusion, immunogold labeling of apolipoproteins on lipid structures in the lipid-laden enterocytes of patients with ABL and AD is best obtained by freeze substitution and embedding in Lowicryl HM20.

摘要

患有脂蛋白组装和分泌遗传疾病的患者,如无β脂蛋白血症(ABL)或安德森病(AD),其肠道活检组织中含有大量积聚在肠细胞内的脂质。确定脂质积聚的细胞内位点以及脂质与哪些载脂蛋白结合,将有助于识别这些疾病中的缺陷,并进一步阐明脂蛋白正常组装和分泌的机制。然而,超微结构免疫金标记受到这些患者肠细胞中积聚脂质保存不佳的阻碍。我们使用常规电子显微镜(固定和超薄切片)以及三种对富含脂质的肠细胞进行免疫金标记的方法:超薄冷冻切片、低温冷冻置换并包埋于Lowicryl K4M中、超低温冷冻置换并包埋于Lowicryl HM20中,以建立一种用于研究这些患者肠道组织的方案。超薄冷冻切片虽然保留了富含脂质的肠细胞的整体形态,但没有保留脂质含量,载脂蛋白B(ApoB)的免疫金标记出现错位。相比之下,冷冻置换并低温包埋于Lowicryl K4M中似乎能更好地保留脂质和脂蛋白结构;然而,载脂蛋白AI和载脂蛋白B的抗原性似乎都丧失了,无法获得特异性标记。冷冻置换并包埋于Lowicryl HM20中能最好地保留脂质和脂蛋白结构,同时保持载脂蛋白的抗原性。总之,对ABL和AD患者富含脂质的肠细胞中脂质结构上的载脂蛋白进行免疫金标记,最好的方法是冷冻置换并包埋于Lowicryl HM20中。

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