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Identification of differentially expressed genes in anagen dermal papilla by suppression subtractive hybridization

机译:抑制性消减杂交鉴定毛发生长乳头中差异表达的基因

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摘要

Background We constructed a cDNA subtractive library of dermal papilla cells (DPCs) in anagen with suppression subtractive hybridization (SSH) technique and clone differentially expressed genes related to DPCs in anagen. Methods Total mRNA was isolated from DPCs of anagen and telogen follicles. Moreover, single-strand (ss) and double-strand (ds) cDNAs were synthesized in turn using SMART PCR cDNA synthesis technology. ds cDNAs then were digested with Rsa I and divided into two groups, and ligated to the specific adaptor 1 and adaptor 2R, respectively. After cDNAs were hybridized with each other twice and underwent two rounds of nested PCR. PCR products were ligated with arms of T/A plasmid vectors to set up the subtractive library. Selected clones were demonstrated by reverse Northern blot and sequenced. The acquired sequence data were aligned against the Genbank nucleotide database. Results cDNA subtractive library of DPCs in anagen follicles was set up successfully with high subtractive efficiency. Thirty-five genes were identified in this study with 22 known functional genes and 13 unknown functional genes. Conclusions All results confirm the effectiveness and sensitivity of SSH in detecting differentially expressed genes from a small amount of clinical samples. Information about such alterations in gene expression could be useful for elucidating the genetic events in hair follicle growth regulation.
机译:背景技术我们采用抑制消减杂交(SSH)技术在生长期建立了真皮乳头细胞(DPC)的cDNA消减文库,并在生长期中克隆了与DPC相关的差异表达基因。方法从毛囊和端粒卵泡的DPCs中分离总mRNA。此外,使用SMART PCR cDNA合成技术依次合成了单链(ss)和双链(ds)cDNA。然后用Rsa I消化ds cDNA并分成两组,并分别连接至特异性衔接子1和衔接子2R。 cDNA相互杂交两次后,进行两轮嵌套式PCR。将PCR产物与T / A质粒载体的臂连接以建立扣除文库。通过反向Northern印迹证实选择的克隆并测序。将获得的序列数据与Genbank核苷酸数据库进行比对。结果成功建立了毛囊中DPCs的cDNA消减文库,消减效率高。在这项研究中鉴定了35个基因,其中22个已知功能基因和13个未知功能基因。结论所有结果都证实了SSH在检测少量临床样品中差异表达基因中的有效性和敏感性。有关基因表达中此类变化的信息可能有助于阐明毛囊生长调节中的遗传事件。

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