Effects of FGF2 and TGFbeta1 on the differentiation of human dental pulp stem cells in vitro

Two crucial growth factors, FGF2 and TGFbeta1, were investigated in this study to determine their inductive effects on the odontoblastic differentiation of human dental pulp stem cells (DPSCs) in vitro. DPSCs were isolated by immunomagnetic bead selection using the STRO-1 antibody, and then co-cultured respectively with FGF2, TGFbeta1 and FGF2+TGFbeta1. The results showed that FGF2 can exert a significant effect on the cell proliferation, while TGFbeta1 or FGF2+TGFbeta1 can initiate an odontoblast-like differentiation of DPSCs. Moreover, FGF2 can synergistically upregulate the effects of TGFbeta1 on the odontoblastic differentiation of DPSCs, as indicated by the increased alkaline phosphatase activity, the polarized cell appearance and secretary ultrastructural features, the formation of mineralized nodules and the gene/protein expression of dentin sialoprotein and dentin matrix protein-1. Together, FGF2 acted primarily on the cell proliferation, while TGFbeta1 and FGF2+TGFbeta1 mainly stimulated the odontoblastic differentiation of DPSCs. This study provides interesting progress in the odontoblastic differentiation of DPSCs induced by FGF2 and TGFbeta1.     

Differential expression of the HMGN family of chromatin proteins during ocular development

The HMGN proteins are a group of non-histone nuclear proteins that associate with the core nucleosome and alter the structure of the chromatin fiber. We investigated the distribution of the three best characterized HMGN family members, HMGN1, HMGN2 and HMGN3 during mouse eye development. HMGN1 protein is evenly distributed in all ocular structures of 10.5 days post-coitum (dpc) mouse embryos however, by 13.5dpc, relatively less HMGN1 is detected in the newly formed lens fiber cells compared to other cell types. In the adult, HMGN1 is detected throughout the retina and lens, although in the cornea, HMGN1 protein is predominately located in the epithelium. HMGN2 is also abundant in all ocular structures of mouse embryos, however, unlike HMGN1, intense immunolabeling is maintained in the lens fiber cells at 13.5dpc. In the adult eye, HMGN2 protein is still found in all lens nuclei while in the cornea, HMGN2 protein is mostly restricted to the epithelium. In contrast, the first detection of HMGN3 in the eye is in the presumptive corneal epithelium and lens fiber cells at 13.5dpc. In the lens, HMGN3 remained lens fiber cell preferred into adulthood. In the cornea, HMGN3 is transiently upregulated in the stroma and endothelium at birth while its expression is restricted to the corneal epithelium in adulthood. In the retina, HMGN3 upregulates around 2 weeks of age and is found at relatively high levels in the inner nuclear and ganglion cell layers of the adult retina. RT-PCR analysis determined that the predominant HMGN3 splice form found in ocular tissues is HMGN3b which lacks the chromatin unfolding domain although HMGN3a mRNA is also detected. These results demonstrate that the HMGN class of chromatin proteins has a dynamic expression pattern in the developing eye.     

赤水桫椤自然保护区土壤甲螨多样性的初步研究

对赤水桫椤自然保护区内旅游点的土壤甲螨进行了调查。调查共获1216号标本,分属31科、43属,其中,盖甲螨属Tectocepheus为优势属。调查区内土壤甲螨的种类多,群落的异质性高,多样性指数高,全区甲螨在MGP分析Ⅰ中为O型,分析Ⅱ中为G型。     

铁过载促进小鼠肝组织发生蛋白质酪氨酸硝化

蛋白质酪氨酸硝化是一种蛋白质翻译后的修饰,其存在会影响酶的催化活性,细胞信号转导和细胞骨架结构．在铁过载情况下,存在引起蛋白质酪氨酸硝化的有利环境,但目前尚无实验证实．本文运用腹腔注射右旋糖苷铁造成小鼠铁过载模型,通过免疫印迹法发现,在铁过载情况下,肝中诱导型一氧化氮合酶表达显著高于正常对照小鼠;铁过载小鼠肝中总体蛋白质硝化程度高于正常小鼠;铁过载引起的蛋白质酪氨酸硝化有一定的选择性,在铁过载小鼠肝中发现一些新的被硝化蛋白质条带（约 57 kD、 35 kD）．上述结果证实,铁过载会促进肝蛋白质酪氨酸硝化．     

酵母亚细胞结构分离效率评估菌株的构建 *

背景: 真核细胞依赖其亚细胞结构高效地完成复杂的生化反应。尽管目前有一些亚细胞结构分离技术,但却缺乏评估这些分离技术的简单、有效方法。目的: 构建可以用来检测亚细胞结构分离效率的酿酒酵母菌株。方法: 通过传统的分子生物学与细胞生物学方法以酿酒酵母为背景构建了亚细胞结构分离效率评估菌株,并进行可行性检测。首先,将酵母各细胞器、自噬体及质膜的标记蛋白进行分组,用不同的蛋白标签分别标记每组蛋白。然后,以标记蛋白-GFP/RFP作为对照组通过免疫荧光法检测蛋白标签对标记蛋白的亚细胞定位是否有影响。最后,通过非连续性密度梯度离心验证该检测菌株能否用来检测亚细胞结构的分离效率。结果: 成功构建了酵母亚细胞结构分离效率评估菌株,该菌株标记了大多数酵母细胞亚细胞结构。挂标签的标记蛋白仍然定位在各自标记蛋白对应的亚细胞结构。非连续性密度梯度离心后,酵母各个亚细胞结构的标记蛋白均可以被检测到。结论: 该酵母亚细胞结构分离效率评估菌株是检测各亚细胞结构分离结果的方便工具,对今后酿酒酵母细胞生物学的研究有潜在的应用价值。     

Fibroblast Activation Protein Overexpression and Clinical Implications in Solid Tumors: A Meta-Analysis

Objective

Fibroblast activation protein (FAP) plays a vital role in tumor invasion and metastasis. Previous studies have reported its prognostic value in different tumors. However, the results of these reports remain controversial. In this study, a meta-analysis was performed to clarify this issue.

Methods

A search of the PubMed, Embase and CNKI databases was conducted to analyze relevant articles. The outcomes included the relations between FAP expression and histological differentiation, tumor invasion, lymph node metastasis, distant metastasis and overall survival (OS). Sensitivity analysis by FAP expression in different cells and tumor types were further subjected to sensitivity analyses as subgroups. Pooled odds ratios (ORs) and hazard ratios (HRs) were evaluated using the random-effects model.

Results

The global analysis included 15 studies concerning various solid tumors. For global analysis, FAP overexpression in tumor tissue displayed significant associations with poor OS and tumor progression (OS: HR = 2.18, P = 0.004; tumor invasion: OR = 4.48, P = 0.007; and lymph node metastasis: OR = 3.80, P = 0.004). The subgroup analyses yielded two notable results. First, the relation between FAP overexpression and poor OS and tumor lymph node metastasis was closer in the patients with FAP expression in tumor cells. Second, the pooled analyses of colorectal cancers or pancreatic cancers all indicated that FAP overexpression was associated with a detrimental OS (HR: 1.72, P = 0.009; HR: 3.18, P = 0.005, respectively). The magnitude of this effect was not statistically significant compared with that in patients with non-colorectal cancers or non-pancreatic cancers. These analyses did not display a statistically significant correlation between FAP expression and histological differentiation and distant metastasis in all of the groups.

Conclusions

FAP expression is associated with worse prognosis in solid tumors, and this association is particularly pronounced if FAP overexpression is found in the tumor cells rather than the stroma.     

KLF8表达修饰及致瘤机制研究进展

KLF8(Krüppel-like factor 8)是Krüppel 样转录因子家族最新成员。KLF8广泛表达于皮肤、脂肪、食道等组织中。早期研究表明,KLF8蛋白具有转录抑制活性,在胚胎发育过程中起重要作用。而近些年大量的研究发现KLF8在多种肿瘤组织中异常高表达,具有转录活化因子活性,可通过对细胞增殖、迁移、侵袭、EMT、细胞干性等多项生理过程调控促进肿瘤发生发展。综述了近年来KLF8研究进展,系统阐述了KLF8表达修饰调控及致瘤机制,为全面深入了解KLF8在肿瘤中作用及后续相关研究提供参考。