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1999年罗伯特·福尔根奖讲座。用于灵敏多靶点DNA和RNA原位杂交的检测与扩增系统:用多彩光谱透视细胞内部

Robert Feulgen Prize Lecture 1999. Detection and amplification systems for sensitive, multiple-target DNA and RNA in situ hybridization: looking inside cells with a spectrum of colors.

作者信息

Speel E J

机构信息

Department of Pathology, University of Zurich, Schmelzbergstrasse 12, CH-8091 Zurich, Switzerland,

出版信息

Histochem Cell Biol. 1999 Aug;112(2):89-113. doi: 10.1007/s004180050396.

DOI:10.1007/s004180050396
PMID:10460463
Abstract

In situ hybridization (ISH) is a powerful technique for localizing specific nucleic acid sequences (DNA, RNA) in microscopic preparations of tissues, cells, chromosomes, and linear DNA fibers. To date, a wide variety of research and diagnostic applications of ISH have been described, making the technique an integral part of studies concerning gene mapping, gene expression, RNA processing and transport, the three-dimensional organization of the nucleus, tumor genetics, microbial infections, and prenatal diagnosis. In this review, I first describe the ISH procedure in short and then focus on the currently available non-radioactive probe-labeling and cytochemical detection methodologies that are utilized to visualize one or multiple different nucleic acid targets in situ with different colors. Special emphasis is placed on the procedures applying fluorescence and brightfield microscopy, the simultaneous detection of nucleic acids and proteins by combined ISH and immunocytochemistry, and, in addition, on the recent progress that has been made with the introduction of signal amplification procedures to increase the detection sensitivity of ISH. Finally, a comparison of fluorescence, enzyme cytochemical, and colloidal gold silver probe detection systems will be presented, and possible future directions of in situ nucleic acid detection will be discussed.

摘要

原位杂交(ISH)是一种在组织、细胞、染色体和线性DNA纤维的显微制片中定位特定核酸序列(DNA、RNA)的强大技术。迄今为止,已经描述了ISH的多种研究和诊断应用,使该技术成为基因图谱绘制、基因表达、RNA加工与运输、细胞核三维组织、肿瘤遗传学、微生物感染及产前诊断等研究中不可或缺的一部分。在本综述中,我首先简要描述ISH程序,然后重点介绍当前可用的非放射性探针标记和细胞化学检测方法,这些方法用于原位以不同颜色可视化一个或多个不同的核酸靶标。特别强调应用荧光和明场显微镜的程序、通过ISH与免疫细胞化学联合同时检测核酸和蛋白质的方法,此外,还强调了引入信号放大程序以提高ISH检测灵敏度方面取得的最新进展。最后,将对荧光、酶细胞化学和胶体金银探针检测系统进行比较,并讨论原位核酸检测未来可能的发展方向。

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1
Robert Feulgen Prize Lecture 1999. Detection and amplification systems for sensitive, multiple-target DNA and RNA in situ hybridization: looking inside cells with a spectrum of colors.1999年罗伯特·福尔根奖讲座。用于灵敏多靶点DNA和RNA原位杂交的检测与扩增系统:用多彩光谱透视细胞内部
Histochem Cell Biol. 1999 Aug;112(2):89-113. doi: 10.1007/s004180050396.
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Cytochemical detection systems for in situ hybridization, and the combination with immunocytochemistry, 'who is still afraid of red, green and blue?'.用于原位杂交的细胞化学检测系统,以及与免疫细胞化学的结合,“谁还怕红、绿、蓝?”
Histochem J. 1995 Nov;27(11):833-58.
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Recent developments in signal amplification methods for in situ hybridization.原位杂交信号放大方法的最新进展。
Diagn Mol Pathol. 2003 Mar;12(1):1-13. doi: 10.1097/00019606-200303000-00001.
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Target and signal amplification: approaches to increase the sensitivity of in situ hybridization.靶标与信号放大:提高原位杂交灵敏度的方法
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In situ hybridization in pathology.病理学中的原位杂交
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Amplification methods to increase the sensitivity of in situ hybridization: play card(s).提高原位杂交灵敏度的扩增方法:发挥作用。 (此译文感觉原英文表述不太清晰准确,翻译可能会稍显生硬,建议进一步确认英文原文的准确意思和应用场景等,以便更精准翻译)
J Histochem Cytochem. 1999 Mar;47(3):281-8. doi: 10.1177/002215549904700302.
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In situ polymerase chain reaction: general methodology and recent advances.原位聚合酶链反应:一般方法及最新进展。
Verh Dtsch Ges Pathol. 1994;78:146-52.
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Tyramide signal amplification (TSA) systems for the enhancement of ISH signals in cytogenetics.用于增强细胞遗传学中ISH信号的酪胺信号放大(TSA)系统。
Curr Protoc Cytom. 2001 May;Chapter 8:Unit 8.9. doi: 10.1002/0471142956.cy0809s11.
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Robert Feulgen Prize Lecture 1995. New approaches to in situ detection of nucleic acids.1995年罗伯特·福尔根奖讲座。核酸原位检测的新方法。
Histochem Cell Biol. 1995 Aug;104(2):81-95. doi: 10.1007/BF01451570.
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The in situ hybridization and immunocytochemistry techniques for characterization of cells expressing specific mRNAs in paraffin-embedded brains.用于鉴定石蜡包埋脑组织中表达特定mRNA的细胞的原位杂交和免疫细胞化学技术。
Brain Res Brain Res Protoc. 1997 May;1(2):195-202. doi: 10.1016/s1385-299x(96)00029-3.

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