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两倍差异是通过实时PCR测定植物中转基因拷贝数的检测限。

Two-fold differences are the detection limit for determining transgene copy numbers in plants by real-time PCR.

作者信息

Bubner Ben, Gase Klaus, Baldwin Ian T

机构信息

Department of Molecular Ecology, Max-Planck-Institute for Chemical Ecology, Hans-Knöll-Str, 8, 07745 Jena, Germany.

出版信息

BMC Biotechnol. 2004 Jul 13;4:14. doi: 10.1186/1472-6750-4-14.

DOI:10.1186/1472-6750-4-14

PMID:15251044

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC493272/

Abstract

BACKGROUND

After transformation, plants that are homozygous and contain one copy of the transgene are typically selected for further study. If real-time PCR is to be used to determine copy number and zygosity, it must be able to distinguish hemizygous from homozygous and one-copy from two-copy plants. That is, it must be able to detect two-fold differences.

RESULTS

When transgenic Nicotiana attenuata plants which had been previously determined by Southern analysis to contain one or two copies of the transgene, were analyzed by real-time PCR (2-delta delta Ct method), the method failed to confirm the results from the Southern analysis. In a second data set we analyzed offspring of a hemizygous one-copy plant, which were expected to segregate into three groups of offspring in a 1:2:1 ratio: no transgene, hemizygous, homozygous. Because it was not possible to distinguish homozygous from hemizygous plants with real-time PCR, we could not verify this segregation ratio.

CONCLUSIONS

Detection of two-fold differences by real-time PCR is essential if this procedure is to be used for the characterization of transgenic plants. However, given the high variability between replicates, a detection of two-fold differences is in many cases not possible; in such cases Southern analysis is the more reliable procedure.

摘要

背景

转化后，通常会选择纯合且含有一份转基因拷贝的植物进行进一步研究。如果要使用实时荧光定量PCR来确定拷贝数和纯合度，它必须能够区分半合子与纯合子，以及单拷贝植物与双拷贝植物。也就是说，它必须能够检测出两倍的差异。

结果

当通过实时荧光定量PCR（2-ΔΔCt法）分析先前经Southern分析确定含有一份或两份转基因拷贝的转基因烟草植株时，该方法未能证实Southern分析的结果。在第二个数据集中，我们分析了一株半合子单拷贝植物的后代，预期这些后代会以1:2:1的比例分成三组：无转基因、半合子、纯合子。由于无法通过实时荧光定量PCR区分纯合子和半合子植物，我们无法验证这种分离比例。

结论

如果要使用实时荧光定量PCR来鉴定转基因植物，检测两倍的差异至关重要。然而，鉴于重复实验之间的高度可变性，在许多情况下无法检测到两倍的差异；在这种情况下，Southern分析是更可靠的方法。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/5b0a/493272/3738fb7c7a61/1472-6750-4-14-1.jpg

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两倍差异是通过实时PCR测定植物中转基因拷贝数的检测限。

Two-fold differences are the detection limit for determining transgene copy numbers in plants by real-time PCR.

作者信息

机构信息

出版信息

BACKGROUND

RESULTS

CONCLUSIONS

背景

结果

结论

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