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Detection of Cross-Sample Contamination in Multiple Myeloma Samples and Sequencing Data.


ABSTRACT: The increasing applicability and sensitivity of next generation sequencing methods exacerbate one of the main issues in the molecular biology laboratory, namely cross-sample contamination. This type of contamination, which could massively increase the rate of false-positive calls in sequencing experiments, can originate at each step during the processing of multiple myeloma samples, such as CD138-selection of tumor cells, RNA and DNA isolation or the processing of sequencing libraries. Here we describe a Droplet Digital PCR (ddPCR) method and a simple bioinformatic solution for the detection of contamination in patient's samples and derived sequencing data, which are based on the same principle: detection of alternative alleles for single-nucleotide polymorphisms (SNPs) that are homozygous according to the control (germ line) sample.

SUBMITTER: Stephens OW 

PROVIDER: S-EPMC9481068 | biostudies-literature | 2018

REPOSITORIES: biostudies-literature

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Detection of Cross-Sample Contamination in Multiple Myeloma Samples and Sequencing Data.

Stephens Owen W OW   Meißner Tobias T   Weinhold Niels N  

Methods in molecular biology (Clifton, N.J.) 20180101


The increasing applicability and sensitivity of next generation sequencing methods exacerbate one of the main issues in the molecular biology laboratory, namely cross-sample contamination. This type of contamination, which could massively increase the rate of false-positive calls in sequencing experiments, can originate at each step during the processing of multiple myeloma samples, such as CD138-selection of tumor cells, RNA and DNA isolation or the processing of sequencing libraries. Here we d  ...[more]

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