A phylo-functional core of gut microbiota in healthy young Chinese cohorts across lifestyles,geography and ethnicities

Structural profiling of healthy human gut microbiota across heterogeneous populations is necessary for benchmarking and characterizing the potential ecosystem services provided by particular gut symbionts for maintaining the health of their hosts. Here we performed a large structural survey of fecal microbiota in 314 healthy young adults, covering 20 rural and urban cohorts from 7 ethnic groups living in 9 provinces throughout China. Canonical analysis of unweighted UniFrac principal coordinates clustered the subjects mainly by their ethnicities/geography and less so by lifestyles. Nine predominant genera, all of which are known to contain short-chain fatty acid producers, co-occurred in all individuals and collectively represented nearly half of the total sequences. Interestingly, species-level compositional profiles within these nine genera still discriminated the subjects according to their ethnicities/geography and lifestyles. Therefore, a phylogenetically diverse core of gut microbiota at the genus level may be commonly shared by distinctive healthy populations as functionally indispensable ecosystem service providers for the hosts.     

猪卵母细胞c-mos基因表达以及RNA干扰

c-mos基因在动物卵母细胞减数分裂调控中起作用,但其作用机制目前仍不清楚。本实验通过RT-PCR、免疫荧光激光共聚焦检测方法检测了猪卵母细胞在体外成熟培养过程中c-mos基因在转录水平、翻译水平上的表达以及蛋白的分布,并应用注射小干扰RNA(siRNA)方法对其进行了RNA干扰(RNAi)研究。结果显示,猪卵母细胞在体外成熟培养过程中c-mos基因mRNA量逐渐增高,电激活后6h接近完全降解;MOS(c-mos基因蛋白产物)在GV卵母细胞生发泡中有一定量的表达,生发泡破裂(GVBD)前表达量增加且开始向卵母细胞胞质弥散,成熟培养44h未成熟卵母细胞中的MOS表达量要高于成熟卵母细胞,激活后6h核区MOS明显减少,但仍然有少量MOS分布于胞质中;成熟培养前干扰c-mos基因,所用三个siRNA都能成功敲低mRNA量,分别是同时期对照组mRNA量的0.08±0.03,0.11±0.06和0.20±0.06倍,干扰后虽然没有完全剔除MOS,但MOS量比同期卵母细胞有明显下降,仍可以引发成熟卵母细胞染色体解凝集。研究结果揭示了猪卵母细胞体外成熟及发育进程中c-mos基因在转录和翻译水平上的动态表达规律,建立了猪卵母细胞c-mos基因RNAi体系,为MOS在猪卵母细胞发育过程中的功能研究建立了重要的基础。     

地衣芽孢杆菌WS-6 β-葡聚糖酶基因的克隆及表达

β-葡聚糖是植物细胞壁中结构性非淀粉多糖,存在于各种饲料农作物中。作为一种抗营养因子,β-葡聚糖使食糜具有很高的粘度,阻碍肠道消化液与食糜的混合,影响营养物质特别是蛋白质和脂肪的消化吸收,降低饲料的利用率。地衣芽孢杆菌分泌的β-葡聚糖酶可分解β-葡聚糖。在青贮发酵过程中,这种酶可降解大麦β-葡聚糖,有效提高家畜、家禽对饲料的利用率。从地衣芽孢杆菌WS-6中克隆到β-1,3-1,4-葡聚糖酶基因并进行测序,将该基因与大肠杆菌表达载体pET32a进行连接,转化大肠杆菌BL21,使该基因得到了有效的表达,为进一步在食品级宿主菌中的表达奠定了基础。     

MicroRNA-129-5p inhibits 3T3-L1 preadipocyte proliferation by targeting G3BP1

MicroRNAs have been regarded to play a crucial role in the proliferation of different cell types including preadipocytes. In our study, we observed that miR-129-5p was down-regulated during 3T3-L1 preadipocyte proliferation, while the expression of G3BP1 showed a contrary tendency. 5-Ethynyl-2′-deoxyuridine (EdU) incorporation assay and flow cytometry showed that overexpression of miR-129-5p could bring about a reduction in S-phase cells and G2-phase arrest. Additional study indicated that miR-129-5p impaired cell cycle-related genes in 3T3-L1 preadipocytes. Importantly, it showed that miR-129-5p directly targeted the 3′UTR of G3BP1 and the expression of G3BP1 was inhibited by miR-129-5p mimic. Moreover, miR-129-5p mimic activated the p38 signaling pathway through up-regulating p38 and the phosphorylation level of p38. In a word, results in our study revealed that miR-129-5p suppressed preadipocyte proliferation via targeting G3BP1 and activating the p38 signaling pathway.     

Adiponectin AS lncRNA inhibits adipogenesis by transferring from nucleus to cytoplasm and attenuating Adiponectin mRNA translation

Adiponectin (AdipoQ) is an adipocyte-derived hormone with positive function on systemic glucose and lipid metabolism. Long noncoding RNA (lncRNA) is emerging as a vital regulator of adipogenesis. However, AdipoQ-related lncRNAs in lipid metabolism have not been explored. Here, AdipoQ antisense (AS) lncRNA was first identified, and we further found that it inhibited adipogenesis. The half-life of AdipoQ AS lncRNA was 10?h, whereas that of AdipoQ mRNA was 4?h. During adipogenic differentiation, AdipoQ AS lncRNA translocated from nucleus to cytoplasm. AdipoQ AS lncRNA and AdipoQ mRNA formed an RNA duplex. Moreover, AdipoQ AS lncRNA delivered via injection of adenovirus expressing AdipoQ AS lncRNA decreases white adipose tissue (WAT), brown adipose tissue (BAT) and liver triglycerides (TG) in mice consuming a high fat diet (HFD). Interestingly, the non-overlapping region of AdipoQ AS lncRNA improved serum glucose tolerance and insulin sensitivity in HFD mice, but not AdipoQ AS lncRNA. In conclusion, AdipoQ AS lncRNA transfer from nucleus to cytoplasm inhibits adipogenesis through formation of an AdipoQ AS lncRNA/AdipoQ mRNA duplex to suppress the translation of AdipoQ mRNA. Taken together, we suggest that AdipoQ AS lncRNA is a novel therapeutic target for obesity-related metabolic diseases.     

MAT2A promotes porcine adipogenesis by mediating H3K27me3 at Wnt10b locus and repressing Wnt/β-catenin signaling

Methionine adenosyltransferase (MAT) is a critical biological enzyme and that can catalyze L-met and ATP to form S-adenosylmethionine (SAM), which is acted as a biological methyl donor in transmethylation reactions involving histone methylation. However, the regulatory effect of methionine adenosyltransferase2A (MAT2A) and its associated methyltransferase activity on adipogenesis is still unclear. In this study, we investigate the effect of MAT2A on adipogenesis and its potential mechanism on histone methylation during porcine preadipocyte differentiation. We demonstrated that overexpression of MAT2A promoted lipid accumulation and significantly up-regulated the levels of adipogenic marker genes including PPARγ, SREBP-1c, and aP2. Whereas, knockdown of MAT2A or inhibition MATII enzyme activity inhibited lipid accumulation and down-regulated the expression of the above-mentioned genes. Mechanistic studies revealed that MAT2A interacted with histone-lysine N-methyltransferase Ezh2 and was recruited to Wnt10b promoter to repress its expression by promoting H3K27 methylation. Additionally, MAT2A interacted with MafK protein and was recruited to MARE element at Wnt10b gene. The catalytic activity of MAT2A as well as its interacting factor-MAT2B, was required for Wnt10b repression and supplying SAM for methyltransferases. Moreover, MAT2A suppressed Wnt10b expression and further inhibited Wnt/β-catenin signaling to promote adipogenesis.     

EP-1不育剂对黑线毛足鼠种群繁殖的影响

为检验EP-1 不育剂对野外鼠类的施用效果,2004 年在内蒙古锡林郭勒盟阿巴嘎旗白音图嘎800 hm² 草场进行了大田实验,并随后进行了逐月的夹线跟踪调查,分析了不育剂(EP-1) 对黑线毛足鼠种群繁殖的效应。结果表明,EP-1 不育剂对黑线毛足鼠种群繁殖的抑制效果良好,投药区与对照区相比,投药区黑线毛足鼠的子宫损伤率达到80% ,平均胎仔数下降到对照区的2 /3 水平,妊娠率也下降到对照区的20% 。但EP-1 不育剂对雄鼠睾丸下降率的作用不明显。一次性投放EP-1 不育剂,对黑线毛足鼠种群的繁殖作用时间可维持4 个月以上,基本可实现对整个繁殖期的控制成效,这可能与黑线毛足鼠具有储藏种子的习性,储藏药饵多次进食有关。     

肝毛细线虫对雌性布氏田鼠繁殖参数的影响

2005年5月,在内蒙古锡林郭勒盟阿巴嘎旗北部,研究了肝毛细线虫(Capillaria hepatica)对典型草原区雌性布氏田鼠(Lasiopodomys brandtii)繁殖参数的影响。采用标准夹线法捕获鼠类,对捕获的鼠类进行常规生物学解剖,根据虫卵有无确定肝毛细线虫病感染情况,记录鼠类名称、体长、体重、胴体重、繁殖特征以及肝毛细线虫病感染情况。由于体重是划分鼠类年龄的常用指标之一,结合布氏田鼠的繁殖特征研究数据,采用25.1~55.0 g之间的雌性个体作为本研究分析样本,并将其分为25.1~35.0 g、35.1~45.0 g和45.1~55.0 g体重(年龄)组。采用卡方检验比较分析同一体重(年龄)组内,肝毛细线虫病感染情况与雌性布氏田鼠妊娠率的关系,T检验分析感染情况与胎仔数的关系。结果显示,在各个体重(年龄)组中,感染肝毛细线虫组布氏田鼠雌鼠妊娠率均略低于未感染组,但感染情况与妊娠情况无显著相关关系(P0.05);感染肝毛细线虫布氏田鼠胎仔数低于未感染布氏田鼠,感染情况与胎仔数有显著相关关系(P0.05)。结果表明,肝毛细线虫病对布氏田鼠妊娠率无明显影响,但对布氏田鼠胎仔数有明显的负面影响。