骨髓样本的常规酸脱钙可保存DNA，用于转移性前列腺癌的荧光原位杂交（FISH）和比较基因组杂交（CGH）研究。

Routine acid decalcification of bone marrow samples can preserve DNA for FISH and CGH studies in metastatic prostate cancer.

作者信息

Brown R S D, Edwards J, Bartlett J W, Jones C, Dogan A

机构信息

Institute of Urology, London, United Kingdom.

出版信息

J Histochem Cytochem. 2002 Jan;50(1):113-5. doi: 10.1177/002215540205000113.

DOI:10.1177/002215540205000113

PMID:11748301

Abstract

Production of paraffin-section material from tissue samples that contain bone requires decalcification. Techniques such as acidic decalcification or EDTA chelation are suitable methods. Acid decalcification is generally quicker than EDTA chelation but studies have suggested that it may result in hydrolysis of DNA. Here we show that limited acid decalcification (less than 24 hr) in 5% formic acid can preserve DNA sufficient for fluorescent in situ hybridization (FISH) or comparative genomic hybridization (CGH) and that prolonged 10% formic acid decalcification results in failure of FISH and only limited retrieval of DNA for CGH studies.

摘要

从含有骨骼的组织样本中制备石蜡切片材料需要进行脱钙处理。酸性脱钙或乙二胺四乙酸（EDTA）螯合等技术是适用的方法。酸性脱钙通常比EDTA螯合更快，但研究表明它可能导致DNA水解。我们在此表明，在5%甲酸中进行有限的酸性脱钙（少于24小时）可以保存足够用于荧光原位杂交（FISH）或比较基因组杂交（CGH）的DNA，而延长的10%甲酸脱钙会导致FISH失败，并且仅能有限地回收用于CGH研究的DNA。

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骨髓样本的常规酸脱钙可保存DNA，用于转移性前列腺癌的荧光原位杂交（FISH）和比较基因组杂交（CGH）研究。

Routine acid decalcification of bone marrow samples can preserve DNA for FISH and CGH studies in metastatic prostate cancer.

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