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从人类存档血浆/血清中分离的DNA的多重链置换扩增:通过焦磷酸测序分析鉴定细胞因子多态性

Multiple strand displacement amplification of DNA isolated from human archival plasma/serum: identification of cytokine polymorphism by pyrosequencing analysis.

作者信息

Sun Yi-Qian, Monstein Hans-Jürg, Ryberg Anna, Borch Kurt

机构信息

Department of Biomedicine and Surgery, University Hospital of Linköping, Sweden.

出版信息

Clin Chim Acta. 2007 Feb;377(1-2):108-13. doi: 10.1016/j.cca.2006.09.003. Epub 2006 Oct 9.

Abstract

BACKGROUND

DNA isolation from formalin-fixed paraffin-embedded tissue appears to be problematic due to degradation caused by fixative. Our aim was to investigate if the isolated genomic DNA from archival plasma/serum, combined with multiple strand displacement amplification (MDA) can be used for genotyping.

METHODS

Nine archival plasma/serum samples and freshly frozen gastric biopsies from the same nine H. pylori-infected subjects were used for DNA isolation. Subsequently, MDA-DNA derived from the plasma/serum samples and DNA isolated from the antrum biopsies were analyzed by PCR amplification and pyrosequencing for the presence of interleukin-1beta gene (IL-1B) single nucleotide polymorphism (SNP). In addition, Southern blot and pyrosequencing analysis of H. pylori-specific PCR amplicons were performed.

RESULTS

IL-1B SNP profiles obtained from the plasma/serum MDA-DNA and antrum biopsy DNA were identical. A C/C genotype was observed in 7 of 9 samples, and 2 of 9 revealed a C/T genotype for IL-1B -511. Similarly, 7 of 9 had a T/T, and 2 of 9 had a C/T genotype for IL-1B -31; 4 of 9 had a C/C, 4 of 9 had a C/T, and 1 of 9 had a T/T genotype, respectively, for IL-1B +3954. Moreover, pyrosequencing analysis revealed the presence of H. pylori 26695 and J99-like 16S rDNA variable V3 region sequence motifs in the antrum biopsies but not in the plasma/serum samples.

CONCLUSIONS

We conclude that MDA combined with pyrosequencing enables a rapid and accurate molecular typing of cytokine single nucleotide polymorphisms from archival plasma/serum samples.

摘要

背景

由于固定剂导致的降解,从福尔马林固定石蜡包埋组织中分离DNA似乎存在问题。我们的目的是研究从存档血浆/血清中分离的基因组DNA与多重链置换扩增(MDA)相结合是否可用于基因分型。

方法

使用来自相同9名幽门螺杆菌感染受试者的9份存档血浆/血清样本和新鲜冷冻的胃活检组织进行DNA分离。随后,通过PCR扩增和焦磷酸测序分析来自血浆/血清样本的MDA-DNA和从胃窦活检组织中分离的DNA,以检测白细胞介素-1β基因(IL-1B)单核苷酸多态性(SNP)的存在。此外,对幽门螺杆菌特异性PCR扩增产物进行了Southern印迹和焦磷酸测序分析。

结果

从血浆/血清MDA-DNA和胃窦活检组织DNA获得的IL-1B SNP谱相同。在9个样本中的7个中观察到C/C基因型,9个样本中的2个显示IL-1B -511为C/T基因型。同样,9个样本中的7个具有T/T基因型,9个样本中的2个具有IL-1B -31的C/T基因型;9个样本中的4个具有C/C基因型,9个样本中的4个具有C/T基因型,9个样本中的1个具有IL-1B +3954的T/T基因型。此外,焦磷酸测序分析显示胃窦活检组织中存在幽门螺杆菌26695和J99样16S rDNA可变V3区域序列基序,但血浆/血清样本中不存在。

结论

我们得出结论,MDA与焦磷酸测序相结合能够对存档血浆/血清样本中的细胞因子单核苷酸多态性进行快速准确的分子分型。

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