体外连续传代对人脐带间充质干细胞分泌组蛋白表型的影响

目的 应用生信分析技术分析不同代次人脐带来源间充质干细胞(human umbilical cord derived mesenchymal stem cells, hUC-MSCs)分泌组蛋白表型差异,探讨体外连续传代对hUC-MSCs分泌组蛋白表型的影响。方法 取第4、6、10、15代(简写为P4、P6、P10、P15)hUC-MSCs的培养上清液,应用高通量人生长因子芯片(QAH-GF-1)、高通量人炎性因子芯片(QAH-INF-3)试剂盒检测80种细胞因子蛋白表达,微阵列数据分析软件Q-Analyzer自动计算出蛋白表达量。将检测浓度最佳置信度占比为50%~100%的蛋白浓度视为质控合格的可靠值,筛选出质控合格的蛋白,应用TBtools 1.105软件绘制层次聚类热图,分析不同代次hUC-MSCs培养上清液中蛋白的表达趋势,记录表达量随体外传代次数增多而增高或降低的蛋白,应用GraphPad Prism 8.0.1软件进行单因素方差分析,以P<0.05为标准筛选出差异表达蛋白,应用在线工具Metascape和微生信进行基因本体(gene ontology, GO)、京都基因与基因组百科全书(Kyoto Encyclopedia of Genes and Genomes, KEGG)富集分析。结果 (1)人炎性因子芯片(QAH-INF-3)中有25种蛋白、人生长因子芯片(QAH-GF-1)中有14种蛋白质控合格。(2)质控合格蛋白的聚类分析结果显示,白细胞介素(interleukin, IL)-6、IL-11、IL-13、IL-17、M-CSF、GM-CSF、TNFR2、Eotaxin-1、MIP-1β、EGFR、SCFR、GDNF、Ⅰ-309、GDF-15、MCP-1及IL-1α共16种蛋白表达随体外扩增代次增加呈逐代下调趋势,IL-7表达随体外扩增代次增加呈逐代上调趋势。(3)P4、P6、P10和P15代hUC-MSCs培养上清液中IL-6、IL-11、IL-13、IL-17、M-CSF、GM-CSF、TNFR2、Eotaxin-1、MIP-1β、EGFR、SCFR、GDNF、Ⅰ-309、GDF-15及MCP-1蛋白表达量比较差异均有统计学意义(P<0.05),IL-1α、IL-7蛋白表达量比较差异均无统计学意义(P>0.05)。P4代hUC-MSCs培养上清液中IL-6、IL-11、IL-13、IL-17、M-CSF、GM-CSF、TNFR2、Eotaxin-1、MIP-1β、EGFR、SCFR、GDNF、Ⅰ-309、GDF-15及MCP-1蛋白表达量均高于P15代hUC-MSCs培养上清液(P<0.05),IL-6、IL-11、IL-13、IL-17、M-CSF、TNFR2、MIP-1β、EGFR、GDNF、Ⅰ-309、GDF-15及MCP-1蛋白表达量均高于P10代hUC-MSCs培养上清液(P<0.05),IL-6、IL-11、IL-13、M-CSF、TNFR2、MIP-1β、EGFR、GDNF、Ⅰ-309蛋白表达量均高于P6代hUC-MSCs培养上清液(P<0.05)。P6代hUC-MSCs培养上清液中IL-6、IL-11、IL-13、GM-CSF、TNFR2、Eotaxin-1、EGFR、SCFR、GDNF和Ⅰ-309蛋白表达量均高于P15代hUC-MSCs培养上清液(P<0.05),TNFR2、GDNF蛋白表达量均高于P10代hUC-MSCs培养上清液(P<0.05)。P10代hUC-MSCs培养上清液中IL-6、IL-11、IL-13、GM-CSF、GDNF和Ⅰ-309蛋白表达量均高于P15代hUC-MSCs培养上清液(P<0.05)。(4)GO富集分析显示,15种差异表达蛋白主要在信号受体激活剂的活性、细胞因子介导的信号通路、细胞迁移的正向调节、生长因子活性等条目中富集。(5)KEGG通路富集分析结果显示,15种差异表达蛋白高富集于细胞因子受体的相互作用、病毒蛋白与细胞因子和细胞因子受体的相互作用、类风湿性关节炎以及IL-17和JAK-STAT信号通路等。结论 体外连续传代可导致hUC-MSCs分泌组蛋白表型变化,表现为高代次hUC-MSCs生长、分化、修复、免疫调节和趋化能力减弱,促炎和衰老表型增加。

Modification in Media Composition to Obtain Secretory Production of STxB-based Vaccines using Escherichia coli

Shiga toxin B-subunit （STxB） from Shigella dysenteriae targets in vivo antigen to cancer cells, dendritic cells （DC） and B cells, which preferentially express the globotriaosylceramide （Gb3） receptor. This pivotal role has encouraged scientists to investigate fusing STxB with other clinical antigens. Due to the challenges of obtaining a functional soluble form of the recombinant STxB, such as formation of inclusion bodies during protein expression, scientists tend to combine STxB with vaccine candidates rather than using their genetically fused forms. In this work, we fused HPV16 E7 as a vaccine candidate to the recombinantly-produced STxB. To minimize the formation of inclusion bodies, we investigated a number of conditions during the expression procedure. Then various strategies were used in order to obtain high yield of soluble recombinant protein from E. coli which included the use of different host strains, reduction of cultivation temperature, as well as using different concentrations of IPTG and different additives （Glycin, Triton X-100, ZnC12）. Our study demonstrated the importance of optimizing incubation parameters for recombinant protein expression in E. coli; also showed that the secretion production can be achieved over the course of a few hours when using additives such as glycine and Triton X-100. Interestingly, it was shown that when the culture mediums were supplemented by additives, there was an inverse ratio between time of induction （TOI） and the level of secreted protein at lower temperatures. This study determines the optimal conditions for high yield soluble E7-STxB expression and subsequently facilitates reaching a functionally soluble form of STxB-based vaccines, which can be considered as a potent vaccine candidate for cervical cancer.