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The mechanism study of miR‐125b in occurrence and progression of multiple myeloma

机译：miR-125b在多发性骨髓瘤发生和发展中的机制研究

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Although many efforts have contributed to improve our knowledge of molecular pathogenesis about multiple myeloma (MM), the role and significance of microRNAs and long noncoding RNAs in MM cells, along with the core mechanism remains virtually absent. The mRNA levels of miR‐125b and MALAT1 in MM cell lines were detected by qRT‐PCR. The influence of Lenti‐Sh‐miR‐125b on cell viability and the Notch‐1 pathway‐related proteins were assessed by MTT method and western blot, respectively. We also investigated the regulation effect between MALAT1 and Notch1 pathway. Moreover, the connection between Notch1 signaling and MM cell growth was discussed in‐depth. The reverse effect of pcDNA‐Notch1 on the cell viability and Notch‐1 pathway proteins induced by Si‐MALAT1 was also studied. Furthermore, miR‐125b overexpressing MM cell lines were injected subcutaneously into nude mice. MiR‐125b and MALAT1 were inversely expressed in style="fixed-case">MM cell lines. Lenti‐Sh‐miR‐125b inhibited the expression of style="fixed-case">MALAT1 and Notch‐1 protein. Binding sites were confirmed between miR‐125b and style="fixed-case">MALAT1, and silencing style="fixed-case">MALAT1 did not alter the expression of Notch‐1. The apoptosis rate was increased and the survival rate was decreased obviously in style="fixed-case">GSI XII (targeted cleavage of Notch‐1 receptor) group, along with the inhibited Notch1 and style="fixed-case">HES1 proteins. Moreover, the decreased cell viability and Notch‐1 pathway proteins induced by Si‐ style="fixed-case">MALAT1 could be reversed by pc style="fixed-case">DNA‐Notch1. Lenti‐Sh‐miR‐125b promoted survival and decreased Notch1 and style="fixed-case">HES1 proteins levels, while this effect was reversed by si ‐ style="fixed-case">MALAT1. MiR‐125b regulated style="fixed-case">MALAT1 expression via Notch1 signaling pathway to regulate cell growth, thus participating in the occurrence and progression of style="fixed-case">MM, which functioned as a therapeutic target for tracking MM.

机译：尽管为提高我们对多发性骨髓瘤（MM）的分子发病机制的了解做出了许多努力，但实际上仍然缺少MM细胞中的microRNA和长非编码RNA的作用和意义以及核心机制。通过qRT-PCR检测MM细胞系中miR-125b和MALAT1的mRNA水平。 Lenti-Sh-miR-125b对细胞活力和Notch-1途径相关蛋白的影响分别通过MTT法和Western blot评估。我们还研究了MALAT1和Notch1途径之间的调节作用。此外，深入讨论了Notch1信号传导与MM细胞生长之间的联系。还研究了pcDNA-Notch1对Si-MALAT1诱导的细胞活力和Notch-1途径蛋白的反向作用。此外，将miR-125b过表达的MM细胞系皮下注射到裸鼠中。 MiR-125b和MALAT1在 style =“ fixed-case”> MM 细胞系中反向表达。 Lenti‐Sh‐miR‐125b抑制 style =“ fixed-case”> MALAT 1和Notch-1蛋白的表达。确认了miR-125b和 style =“ fixed-case”> MALAT 1之间的结合位点，而 style =“ fixed-case”> MALAT 1沉默并没有改变其表达。缺口-1。 Notch-1受体的靶向裂解 style =“ fixed-case”> GSI XII 组细胞凋亡率增加，存活率明显降低，Notch1和 style = “ fixed-case”> HES 1蛋白。此外，pc style =“ fixed-case”> MAL 可以逆转由Si- style =“ fixed-case”> MALAT 1诱导的细胞活力和Notch-1通路蛋白的降低跨度>-缺口1。 Lenti‐Sh‐miR‐125b促进存活并降低Notch1和 style =“ fixed-case”> HES 1蛋白水平，而si ‐ style =“ fixed-case”> MALAT 1。 MiR-125b通过Notch1信号通路调节 style =“ fixed-case”> MALAT 1表达以调节细胞生长，从而参与 style =“ fixed-case”> MM < / span>，作为追踪MM的治疗目标。

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期刊名称 Cancer Medicine
作者
Da Gao; Zhen Xiao; Hui‐Ping Li; Dong‐Hai Han; Ya‐Peng Zhang;
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作者单位

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年(卷),期 2018(7),1
年度 2018
页码 134–145
总页数 12
原文格式 PDF
正文语种
中图分类肿瘤学;
关键词
lncRNA MALAT1 MiR‐125b multiple myeloma notch‐1 pathway;

机译：lncRNA MALAT1;MiR-125b;多发性骨髓瘤;Notch-1途径;
入库时间 2022-08-21 11:02:06

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专利

1. The mechanism study of miR‐125b in occurrence and progression of multiple myeloma [J] . Da Gao, Zhen Xiao, Hui‐Ping Li, Cancer Medicine . 2017,第1期

机译：miR-125b在多发性骨髓瘤发生和发展中的机制研究
2. Systematic analysis of berberine-induced signaling pathway between miRNA clusters and mRNAs and identification of mir-99a similar to 125b cluster function by seed-targeting inhibitors in multiple myeloma cells [J] . Feng Maoxiao, Luo Xiaochuang, Gu Chunming, RNA biology . 2015,第1期

机译：小ber碱诱导的miRNA簇与mRNA之间的信号转导途径的系统分析和种子靶向抑制剂在多发性骨髓瘤细胞中鉴定类似于125b簇功能的mir-99a
3. Systematic analysis of berberine-induced signaling pathway between miRNA clusters and mRNAs and identification of mir-99a similar to 125b cluster function by seed-targeting inhibitors in multiple myeloma cells [J] . Feng Maoxiao, Luo Xiaochuang, Gu Chunming, RNA biology . 2015,第1期

机译：在多发性骨髓瘤细胞中靶向抑制剂与MiR-99a与MiR-99a相似的MiR-99a鉴定的系统分析
4. Bioinformatics Analysis for Evaluation of the Diagnostic Potentialities of miR-19b, -125b and -205 as Liquid Biopsy Markers of Prostate Cancer [C] . O. E. Bryzgunova, E. A. Lekchnov, M. M. Zaripov, International Conference on Physics of Cancer : Interdisciplinary Problems and Clinical Applications . 2017

机译：生物信息学分析MiR-19B，-125b和-205诊断潜力作为前列腺癌的液体活组织检查标志物
5. A study of microRNAs associated with multiple myeloma pathogenesis and microRNAs/TP53 feedback circuit in human cancers, multiple myeloma and glioblastoma multiforme. [D] . Suh, Sung-Suk. 2012

机译：在人类癌症，多发性骨髓瘤和多形性胶质母细胞瘤中与多发性骨髓瘤发病机制相关的microRNA和microRNA / TP53反馈回路的研究。
6. Systematic analysis of berberine-induced signaling pathway between miRNA clusters and mRNAs and identification of mir-99a∼125b cluster function by seed-targeting inhibitors in multiple myeloma cells [O] . Maoxiao Feng, Xiaochuang Luo, Chunming Gu, 2015

机译：小ber碱诱导的miRNA簇与mRNA之间的信号转导途径的系统分析和种子靶向抑制剂在多发性骨髓瘤细胞中鉴定mir-99a〜125b簇的功能
7. The mechanism study of miR-125b in occurrence and progression of multiple myeloma [O] . Da Gao, Zhen Xiao, Hui-Ping Li, 2017

机译：miR-125b在多发性骨髓瘤发生和进展中的机制研究

The mechanism study of miR‐125b in occurrence and progression of multiple myeloma

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