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两种棘球绦虫原头节促进骨髓间充质干细胞钙化的差异性分析 被引量:3
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作者 桂显伟 姜慧娇 +7 位作者 武杰 梁学奇 徐小丹 王二强 邹海亮 陈贺捷 陈雪玲 吴向未 《中国组织工程研究》 CAS 北大核心 2021年第1期38-43,共6页
背景:细粒棘球蚴与泡状棘球蚴的生长方式不同,肝细粒棘球蚴病可以形成完整的纤维钙化囊壁,肝泡状棘球蚴病呈浸润性生长,不能形成完整的纤维钙化囊壁。骨髓间充质干细胞参与棘球蚴病纤维钙化囊壁的形成,但细粒棘球蚴和泡状棘球蚴钙化特... 背景:细粒棘球蚴与泡状棘球蚴的生长方式不同,肝细粒棘球蚴病可以形成完整的纤维钙化囊壁,肝泡状棘球蚴病呈浸润性生长,不能形成完整的纤维钙化囊壁。骨髓间充质干细胞参与棘球蚴病纤维钙化囊壁的形成,但细粒棘球蚴和泡状棘球蚴钙化特征不同与骨髓间充质干细胞的作用尚不清楚。目的:比较2种棘球绦虫原头节对骨髓间充质干细胞钙化的作用,初步探讨2种棘球蚴钙化灶差异的形成机制。方法:提取、培养、鉴定C57BL/6小鼠骨髓间充质干细胞。将骨髓间充质干细胞分别与泡状棘球绦虫原头节、细粒棘球绦虫原头节共培养,以骨髓间充质干细胞单独培养为对照组。共培养1,4,7 d取骨髓间充质干细胞通过微量酶标法检测成骨标记物碱性磷酸酶活性,RT-qPCR检测BMP2和RUNX2 mRNA的表达,Western blot检测BMP2、RUNX2和P-Smad1/5/8的蛋白表达。结果与结论:①细粒棘球绦虫原头节共培养组、泡状棘球绦虫原头节共培养组1,4 d的碱性磷酸酶活性均高于对照组(P <0.05),且细粒棘球绦虫原头节共培养组1,4,7 d的碱性磷酸酶活性高于泡状棘球绦虫原头节共培养组(P <0.05)。②Western blot结果显示:细粒棘球绦虫原头节共培养组和泡状棘球绦虫原头节共培养组1,4 d的BMP2、RUNX2、P-Smad1/5/8蛋白表达高于对照组(P <0.05),细粒棘球绦虫原头节共培养组高于泡状棘球绦虫原头节共培养组(P <0.05)。③RT-qPCR结果显示:细粒棘球绦虫原头节共培养组1,4,7 d的BMP2、RUNX2mRNA表达水平显著高于对照组(P <0.05),细粒棘球绦虫原头节共培养组4,7 d的BMP2、RUNX2 mRNA表达水平显著高于泡状棘球绦虫原头节共培养组(P <0.05)。泡状棘球绦虫原头节共培养组1,4,7 d的RUNX2 mRNA表达水平显著高于对照组(P <0.05)。④结果表明,棘球绦虫原头节与骨髓间充质干细胞共培养通过上调BMP-Smad1/5/8通路促进骨髓间充质干细胞钙化因子碱性磷酸酶和RUNX2的表达,共培养后期泡状棘球蚴促钙化作用明显减弱,细粒棘球蚴促钙化作用保持不变,提示该机制可能与2种棘球蚴生长方式不同相关。 展开更多
关键词 骨髓间充质干细胞 泡状 细粒 钙化 纤维钙化囊壁 棘球绦虫原头节
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Construction and primary characterization of Echinococcus multilocularis protoscolex cDNA expression library
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作者 李淑萍 陈雅棠 《Chinese Medical Journal》 SCIE CAS CSCD 2001年第2期12-15,103,共5页
Objective To construct a λgt11 cDNA expression library of Echinococcus multilocularis protoscolex isolated in China. Methods Echinococcus multilocularis protoscolex mRNA was extracted using a Quickprep MicromRNA pu... Objective To construct a λgt11 cDNA expression library of Echinococcus multilocularis protoscolex isolated in China. Methods Echinococcus multilocularis protoscolex mRNA was extracted using a Quickprep MicromRNA purification kit based on combining of the disruptive and protective properties of guanidinium thiocyanate (GTC) with the speed and selectivity of oligo (dT)-cellulose chromatography in a spum-column with some modification. Purified mRNA (1.8 μg) was submitted to reverse transcription using random hexamers [pd(N6)]. The double-strand blunt-ended cDNAs were ligated with an EcoRI/NotI adaptor to form a cohesive EcoRI end. Subsequently the synthesized cDNA was inserted into vector λgt11 EcoRI arms. After being packaged in vitro, λgt11 was put to an infectious bacteria Echinococcus coli (E.coli) strain Y1090; the recombinants were screened by color selection. PCR amplification was performed to evaluate the size of insertion DNA fragments.Results The recombinant ratio was nearly 100% and approximately 1×106 clones could be derived from this λgt11 cDNA library. PCR results indicated that the insertion DNAs were about 1.48 kb. Conclusions A λgt11 cDNA expression library consisting of a million recombinant clones has been constructed from Echinococcus multicularis protoscolex mRNA. Further studies on this library are deserved. 展开更多
关键词 echinococcus multicularis · protoscolex λgt11 cDNA library clone
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