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在常规处理的皮肤病理学标本中检测特定的信使核糖核酸

Detection of specific mRNAs in routinely processed dermatopathology specimens.

作者信息

Tyrrell L, Elias J, Longley J

机构信息

Yale University School of Medicine, Department of Dermatology, New Haven, CT 06520-8059, USA.

出版信息

Am J Dermatopathol. 1995 Oct;17(5):476-83. doi: 10.1097/00000372-199510000-00008.

DOI:10.1097/00000372-199510000-00008
PMID:8599453
Abstract

To determine the effect of different fixatives on the recovery and detection of mRNAs from archival histopathology specimens, biopsies of normal skin were fixed in neutral and alcohol-buffered formalin, acetone, Carnoy's fixative, methacarn, and Bouin's solution. Tissue was routinely processed, and sections were either mounted for in situ hybridization or deparaffinized for RNA extraction. Extracted mRNA was reverse-transcribed using random hexamers, and the resulting cDNA was amplified by the polymerase chain reaction using primers specific for glyceraldehyde-3-phosphate dehydrogenase (GAPDH) and beta-actin. Amplification products of both GAPDH and actin could be detected by gel electrophoresis from tissues processed in all fixatives except Bouin's. A parallel study of formalin-fixed, paraffin-embedded archival biopsies accessioned since 1990 gave similar results. Less abundant mRNAs, such as those encoding interleukin-11 or the T-cell receptor beta-chain, could be detected by Southern blotting and hybridization with labeled oligonucleotide probes or by cloning and sequencing. In situ hybridization studies using oligonucleotide probes were most successful with tissue fixed in formalin, including both the experimentally fixed tissues and the archival biopsy samples. Thus, mRNAs may be isolated from and localized in formalin-fixed, paraffin-embedded archival material. Because dermatopathology laboratory archives typically contain samples from a wide spectrum of diseases that can be accessed without Human Investigation Committee approval, these laboratories represent a logical starting point for studying gene regulation and expression in skin.

摘要

为了确定不同固定剂对存档组织病理学标本中mRNA的回收和检测的影响,将正常皮肤活检组织固定于中性和酒精缓冲甲醛、丙酮、卡诺固定液、甲醇冰醋酸固定液及波因液中。组织经常规处理,切片用于原位杂交或脱蜡以进行RNA提取。提取的mRNA使用随机六聚体进行逆转录,所得cDNA使用针对甘油醛-3-磷酸脱氢酶(GAPDH)和β-肌动蛋白的引物通过聚合酶链反应进行扩增。除波因液处理的组织外,在所有固定剂处理的组织中,通过凝胶电泳均可检测到GAPDH和肌动蛋白的扩增产物。对1990年以来接收的福尔马林固定、石蜡包埋的存档活检组织进行的平行研究也得到了类似结果。丰度较低的mRNA,如编码白细胞介素-11或T细胞受体β链的mRNA,可通过Southern印迹法和与标记寡核苷酸探针杂交或通过克隆和测序进行检测。使用寡核苷酸探针的原位杂交研究在福尔马林固定的组织中最为成功,包括实验固定的组织和存档活检样本。因此,mRNA可从福尔马林固定、石蜡包埋的存档材料中分离并定位。由于皮肤病理学实验室档案通常包含无需人类研究委员会批准即可获取的各种疾病样本,这些实验室是研究皮肤基因调控和表达的合理起点。

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Detection of specific mRNAs in routinely processed dermatopathology specimens.在常规处理的皮肤病理学标本中检测特定的信使核糖核酸
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