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Development of a multiplex quantitative fluorescent PCR assay for identification of rearrangements in the AZFb and AZFc regions

机译:开发用于鉴定AZFb和AZFc区重排的多重定量荧光PCR检测方法

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摘要

The azoospermia factor b (AZFb) and azoospermia factor c (AZFc) regions in the human Y chromosome consist of five palindromes constructed from six distinct families of amplicons and are prone to rearrangement. Partial deletion and duplication in the region can cause azoospermia or oligozoospermia and male infertility. The aim of the study was to establish a quantitative fluorescent PCR (QF-PCR) assay to classify AZFb and AZFc rearrangements. A single pair of fluorescent primers was designed to amplify simultaneously the amplicon in AZFc and the length-variant homologous sequences outside of the region as control. Since the copy number of the control sequences is fixed in the human genome, dosage of the target could be easily obtained through comparing the height of the fluorescent peaks between the target and the control after amplification with limited PCR cycles. Most types of rearrangements in AZFb and AZFc regions could be classified with QF-PCR containing four such primer pairs. Eleven types of rearrangement in AZFb and AZFc regions were well discriminated with QF-PCR. In conclusion, QF-PCR is a simple and reliable method to detect rearrangements in AZFb and AZFc.
机译:人Y染色体中的无精症因子b(AZFb)和无精症因子c(AZFc)区由六个不同的扩增子家族构成的五个回文质组成,并且易于重排。该区域的部分缺失和重复可导致无精症或少精症和男性不育。该研究的目的是建立定量荧光PCR(QF-PCR)分析以对AZFb和AZFc重排进行分类。设计一对荧光引物以同时扩增AZFc中的扩增子和该区域外的长度变异同源序列作为对照。由于控制序列的拷贝数在人类基因组中是固定的,因此通过在有限的PCR循环中扩增后,通过比较靶标和对照之间的荧光峰的高度,可以轻松获得靶标的剂量。可以使用包含四个此类引物对的QF-PCR对AZFb和AZFc区中的大多数类型的重排进行分类。用QF-PCR可以很好地区分AZFb和AZFc区的11种重排类型。总之,QF-PCR是检测AZFb和AZFc中重排的一种简单可靠的方法。

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