泌体研究策略与方法.pptx
单击此处编辑母版标题样式,单击此处编辑母版文本样式,第二级,第三级,第四级,第五级,2020/3/26,#,外泌体研究策略,目录,一、外泌体概述,二、外泌研究兴起,三、外泌体基础研究技术,四、外泌体研究策略基本逻辑,五、外泌体研究实例,外泌体概述,Exosome,是直径约为,30-150nm,,密度在,1.13-1.21g/m1,的小囊泡。,Exosome,天然存在于体液中,包括血液、唾液、尿液和母乳,外泌体,(Exosome),是活细胞分泌的来源于晚期核内体,(,也称为多囊泡体,),的膜性囊泡。,Tan A Advanced drug delivery reviews,2013,65(3):357-367.,外泌体研究的兴起,2018,外泌体中标项目研究的主要癌症种类,2018,外泌体中标项目机制研究涉及的主要非编码,RNA,种类,2018,外泌体中标项目的主要外泌体来源,外泌体研究基础技术,1,、外泌体分离,1,),超速离心,2,),磁珠免疫捕获,3,),沉淀或过滤法,,2,、外泌体鉴定与定量,1,)鉴定:,电镜,或,NTA,来分析其大小和形态,,,流式细胞仪,或,WB,检测,表面标记,蛋白,,Western blot,和,ELISA,检测,TSG101,、,CD63,。,2,)定量:,NTA,检测外泌体数量,,BCA,定量检测蛋白浓度。,3,、外泌体功能研究,1,)荧光标记外泌体检测外泌体进入细胞,2,)常规实验:外泌体处理细胞检测功能,3,),WB/qPCR/,荧光标记技术检测外泌体中发挥关键作用的生物分子在受体细胞胞核、胞质以及外泌体中的表达。,外泌体研究策略基本逻辑,Journal of Hematology&Oncology,December 2015,8:83,外泌体研究的本质:供体细胞对受体细胞的功能影响,通过外泌这个介质发挥作用,外泌体研究基本路线图,相互作用的受,/,供体细胞的选择,供体细胞外泌体分离和鉴定,外泌体对受体细胞功能的影响,外泌体能够影响受体细胞功能的因素:细胞因子、,mRNA,、,lncRNA,、,miRNA,、,circRNA,以及其他。,外泌体研究整体研究策略,1,、通常来说只要是涉及到两种不同细胞甚至同一种细胞的两种不同状态:癌与正常细胞(癌转化与抑制)、干细胞与高分化细胞损伤与修复)以及功能状态细胞与非激活状态细胞,就可以设计外泌体研究方案。,2,、外泌体研究关键点:,参与外泌功能的关键生物分子,细胞因子、,mRNA,、,lncRNA,、,miRNA,、,circRNA,以及其他。,3,、外泌体设计基本思路有:关键生物分子到外泌体或外泌体到关键生物分子。但无论怎样其核心无法改变一定或有效应受体(供体有时会忽略,例如血清来源外泌体等,实例一 由生物分子到外泌体,Exosome-Transmitted lncARSR Promotes Sunitinib,Resistance in Renal Cancer by Acting as a,Competing Endogenous RNA,1,、,lncARSR Is Highly Expressed in Sunitinib-Resistant RCC Cells,2,、,lncARSR Is Modulated by AKT/FOXO Axis in Sunitinib-Resistant RCC Cells,3,、,lncARSR Is Required for Sunitinib Resistance of RCC,4,、,lncARSR Levels in Plasma and Tumor Tissues Correlate with Sunitinib Response in RCC Patients,5,、,Packaging of lncARSR into Exosomes Is Mediated by hnRNPA2B1,6,、,Intercellular Transfer of lncARSR by Exosomes Disseminates Sunitinib Resistance,7,、,AXL and c-MET Are Responsible for lncARSR-Mediated Sunitinib Resistance,8,、,lncARSR Functions as a ceRNA for miR-34 and miR-449 to Facilitate AXL and c-MET Expression,9,、,Targeting lncARSR Restores Sunitinib Response in RCC,总结:,这篇文章中外泌体不是主角,外泌体只是作为长非编,RNA,功能作用机制的一个重要方面,但总体上给我们展现了外泌体研究的一系列重要方法:,1,)外泌体功能探讨的基础:供体细胞(舒尼替尼抗性肾癌细胞),/,受体细胞(舒尼替你敏感性肾癌细胞)。,2,)外泌体功能前期预实验:功能生物分子位于外泌体中(图,5A,)、外泌体电镜检测(图,5B,)、不同来源外泌体中功能分子的差异表达(图,5C,)、功能分子被特异包裹入外泌体的关键蛋白检测(图,5D,)。,3,)外泌体功能实验:外泌体处理细胞、外泌体进细胞核以及受供体细胞共孵育等。,实例二由外泌体到生物分子,Endothelial microparticles mediate inflammation-induced,vascular calcification,1,、,TNF-a up-regulates EC BMP-2 expression through activation of NF-kB and stimulates the generation of EMPs,2,、,Annexin V,calcium,and BMP-2 in EMPs from HUVECs stimulated by TNF-a,BMP-2,表面标记流式检测;,SN50 nf-kb,抑制剂,3,、,The effect of EMPs from HUVECs stimulated by TNF-a on VSMC calcification,A,:,vs.NP;b,:,0.05 vs.HP plus Control-EMP;c,:,vs.HP plus TNF-a EMP.,HP,高磷、,SN,不含外泌体上清,4,、,Knockdown of BMP-2 in HUVECs produces nonmineralizing TNF-a-EMPs,5,、,EMPs from patients with CKD stimulate VSMC calcification and osteogenesis,And from senescent HUVECs induce calcification and osteogenic changes of VSMCs,6,、,Internalization of EMPs by VSMCs,实例三,CD90+liver cancer cells modulate endothelial cell phenotype through the release of exosomes,containing H19 lncRNA,1,、,CD90+cells show a mesenchymal phenotype and actively release exosomes,2,、,Exosomes released by CD90+Huh7 cells affect HUVECs by promoting tube formation and cell-cell adhesion,ICAM-1,细胞粘附因子,3,、,CD90+cells express the lncRNA H19 and release it viaexosomes,4,、,LncRNA H19 stimulates angiogenesis and promotes the adhesion of CD90+Huh7 cells to endothelial cell monolayer,