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显微切割肿瘤细胞的杂合性缺失(LOH)和微卫星不稳定性(MSI)分析中的聚合酶链反应(PCR)假象

PCR artifacts in LOH and MSI analysis of microdissected tumor cells.

作者信息

Sieben N L, ter Haar N T, Cornelisse C J, Fleuren G J, Cleton-Jansen A M

机构信息

Department of Pathology, University Medical Center, Leiden, The Netherlands.

出版信息

Hum Pathol. 2000 Nov;31(11):1414-9.

Abstract

Polymerase chain reaction (PCR) analysis to study loss of heterozygosity (LOH) and microsatellite instability (MSI) in tumors is widely used. Microdissection techniques are applied to obtain tumor-specific tissue cells. By microdissection, however, the amount of template DNA extracted may vary considerably and interfere with optimal PCR amplification. To circumvent LOH and MSI misinterpretations due to low DNA input, we have assessed the critical level of DNA input for reliable PCR analysis. PCR analysis was performed by using 18 polymorphic markers (mono-, di-, tri-, and tetranucleotide) on DNA derived from both paraffin-embedded, formalin-fixed, and fresh frozen tumor specimens at template input levels ranging from 0.05 to 25.0 ng. We show a highly significant relation between DNA input and the occurrence of LOH and MSI artifacts. Furthermore, for DNA extracted from paraffin-embedded material, the percentage of LOH artifacts is significantly higher compared with DNA extracted from frozen tissue. For reliable PCR analyses using a mono-, di-, tri-, or tetranucleotide marker, a minimum of 10.0 ng DNA is required when DNA is isolated from formalin-fixed, paraffin-embedded tissue and 5.0 ng when isolated from fresh frozen tissue. HUM PATHOL 31:1414-1419.

摘要

聚合酶链反应(PCR)分析用于研究肿瘤中的杂合性缺失(LOH)和微卫星不稳定性(MSI),应用广泛。微切割技术用于获取肿瘤特异性组织细胞。然而,通过微切割提取的模板DNA量可能有很大差异,并干扰最佳PCR扩增。为避免因低DNA输入量导致的LOH和MSI误判,我们评估了可靠PCR分析所需的关键DNA输入水平。使用18个多态性标记(单核苷酸、二核苷酸、三核苷酸和四核苷酸)对来自石蜡包埋、福尔马林固定和新鲜冷冻肿瘤标本的DNA进行PCR分析,模板输入水平范围为0.05至25.0 ng。我们发现DNA输入量与LOH和MSI假象的出现之间存在高度显著的关系。此外,从石蜡包埋材料中提取的DNA产生的LOH假象百分比明显高于从冷冻组织中提取的DNA。对于使用单核苷酸、二核苷酸、三核苷酸或四核苷酸标记进行可靠的PCR分析,从福尔马林固定、石蜡包埋组织中分离DNA时,至少需要10.0 ng DNA,从新鲜冷冻组织中分离时需要5.0 ng DNA。《人类病理学》31:1414 - 1419。

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