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METHOD FOR DETERMINING NUCLEIC ACID DEGRADATION IN A SAMPLE IN WHICH AT LEAST TWO OVERLAPPING AMPLICONS ARE PRODUCED AND TWO PROBES ARE USED IN THE METHOD
METHOD FOR DETERMINING NUCLEIC ACID DEGRADATION IN A SAMPLE IN WHICH AT LEAST TWO OVERLAPPING AMPLICONS ARE PRODUCED AND TWO PROBES ARE USED IN THE METHOD
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机译:确定至少产生两个重叠的样品并使用两个问题的样品中核酸降解的方法
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摘要
The present invention relates to a method for assessing the status of nucleic acid degradation and/or integrity of one or more nucleic acids in a sample, comprising the steps amplifying at least two overlapping regions within at least one locus (e.g. by heminested or nested PCR), and detecting the amount of the at least two amplification products through the use of at least two probes, wherein one probe binds to the region of overlap and the at least one other probe binds to a non-overlapping region. The invention further relates to a method of designing primers and/or probes for amplifying at least two overlapping regions within at least one locus, wherein the locus that is amplified is a single copy locus (SCL) or multicopy locus (MLC). The invention also relates to a primer and a primer pair for amplifying at least two overlapping regions from one nucleic acid template which is a multicopy locus present in 21 loci in the human genome. These primers and probes may be in a kit. Hence, the invention also relates to a kit for assessing the status of nucleic acid degradation and/or integrity of one or more nucleic acids in a sample.
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