MiR-135b调控BMPs/Smads信号通路在牙髓细胞成牙本质向分化中的作用及机制研究
项目来源
广(略)技(略)
项目主持人
宋(略)
项目受资助机构
中(略)�
立项年度
2(略)�
立项时间
未(略)
项目编号
2(略)�A030310227
项目级别
省(略)
研究期限
未(略) (略)
受资助金额
1(略)0(略)
学科
临(略)�
学科代码
未(略)
基金类别
广(略)然(略)金(略)启(略)
关键词
M(略)1(略) (略)m(略) (略)m(略) (略)胞(略);(略)本(略) (略)e(略)d(略)e(略)t(略)i(略);(略)o(略)b(略)t(略)
参与者
未(略)
参与机构
未(略)
项目标书摘要:目的(略)髓细胞(hDPCs(略)的功能。 (略)比较性miRNA微(略)的成牙本质细胞样分(略)达。通过定量实时逆(略)T-PCR)和原位(略)croRNA-13(略))的丰度。生物信息(略)结合,用于鉴定与m(略)的靶标。进行了mi(略)研究hDPC在成牙(略)和机制。通过单因素(略)学生t检验进行统计(略)结果:鉴定了36种(略)胞样分化中差异表达(略)hDPCs分化过程(略)达明显下调(P (略)观察结果表明miR(略)质细胞样hDPC分(略)抑制miR-135(略)工程的有前途的治疗(略)
Applicati(略): Aim:To (略) the func(略)NAs in od(略)ike diffe(略)of human (略) cells(hD(略) Methodo(略)ated comp(略)NA microa(略)ing was u(略)rmine the(略)al miRNAs(略) in odont(略) differen(略)hDPCs.The(略)of microR(略)-135b)was(略)y quantit(略)time reve(略)iptase po(略)ain react(略))and in s(略)zation(IS(略)matic ana(略)ned with (略)assays we(略) to ident(略)gets inte(略)h miR-135(略)ssion of (略)s perform(略)tigate th(略)mechanism(略)last-like(略)ation of (略)stical an(略)performed(略) analysis(略)e(anova)o(略) t-test. (略)lts:Thirt(略)rentially(略)microRNAs(略)last-like(略)ation of (略)identifie(略)expressio(略)ficantly (略)ed during(略)erentiati(略) Conclusi(略)bservatio(略)d a poten(略)f miR-135(略)ing odont(略) differen(略)hDPCs and(略) of miR-1(略)e a promi(略)eutic way(略)ate denti(略)ngineerin(略)
项目受资助省
广(略)
1.MicroRNA 135b通过调节Smad5和Smad4抑制人牙髓细胞成牙本质细胞样分化(MicroRNA-135b inhibits odontoblast-like differentiation of human dental pulp cells by regulating Smad5 and Smad4)
- 关键词:
- MiR-135b、Smad4、Smad5、细胞分化、成牙本质细胞、MiR-135b、Smad4、Smad5、cell differentiation、odontoblasts
- 宋智;
- 《中山大学;》
- 2020年
- 报告
目的:研究miRNA在人牙髓细胞(hDPCs)成牙本质细胞样分化中的功能。 方法:采用集成的比较性miRNA微阵列分析来确定hDPC的成牙本质细胞样分化中的差异miRNA表达。通过定量实时逆转录聚合酶链反应(qRT-PCR)和原位杂交(ISH)测量microRNA-135b(miR-135b)的丰度。生物信息学分析与萤光素酶分析相结合,用于鉴定与miR-135b相互作用的靶标。进行了miR-135b的过表达以研究hDPC在成牙本质细胞样分化中的作用和机制。通过单因素方差分析(方差分析)或学生t检验进行统计分析。 结果:鉴定了36种在hDPC的成牙本质细胞样分化中差异表达的microRNA。在hDPCs分化过程中,MiR-135b表达明显下调(P<0.05)。此外,miR-135b能够与Smad5和Smad4的3'-UTR结合并抑制这两个基因的表达(P<0.05)。此外,miR-135b的过表达抑制了hDPC的成牙本质细胞样分化,并减弱了Smad5和Smad4的表达(P<0.05)。 结论:这些观察结果表明miR-135b在介导成牙本质细胞样hDPC分化中具有潜在作用,并且抑制miR-135b可能是促进牙本质组织工程的有前途的治疗方法。 Aim:To investigate the function of miRNAs in odontoblast-like differentiation of human dental pulp cells(hDPCs). Methodology:Integrated comparative miRNA microarray profiling was used to determine the differential miRNAs expression in odontoblast-like differentiation of hDPCs.The abundance of microRNA-135b(miR-135b)was measured by quantitative real-time reverse transcriptase polymerase chain reaction(qRT-PCR)and in situ hybridization(ISH).Bioinformatic analyses combined with luciferase assays were utilized to identify the targets interacting with miR-135b.Overexpression of miR-135b was performed to investigate the role and mechanism in odontoblast-like differentiation of hDPCs.Statistical analysis was performed by one-way analysis of variance(anova)or Student's t-test. Results:Thirty-six differentially expressed microRNAs in odontoblast-like differentiation of hDPCs were identified.MiR-135b expression was significantly downregulated during hDPCs differentiation(P<0.05).In addition,miR-135b was able to bind to the 3'-UTR of the Smad5 and Smad4 and repressed these two genes expression(P<0.05).Furthermore,overexpression of miR-135b suppressed odontoblast-like differentiation of hDPCs and attenuated the expression of Smad5 and Smad4(P<0.05). Conclusions:These observations indicated a potential role of miR-135b in mediating odontoblast-like differentiation of hDPCs and inhibition of miR-135b might be a promising therapeutic way to facilitate dentine tissue engineering.
...