Physiological and pathological roles of mast cells in adipose tissue

Mast cells are important cells for the innate immunity that reside in tissues including adipose tissue and are involved in various physiological and pathological processes by producing a range of biological mediators. Adipose tissue not only acts as an energy depot and regulator of energy homeostasis that can deposit excess energy and dissipate energy through heat, but also is an active endocrine organ capable of producing hormones and adipokines. The dysfunction of adipose tissue is highly correlated with metabolic disorders, such as obesity, type 2 diabetes mellitus and so on. This review focuses on the physiological and pathological roles of mast cells in adipose tissue.     

大银鱼卵细胞粘丝扫描电镜观察

用扫描电镜观察了大银鱼的第Ⅲ时相，第Ⅳ时相，第Ⅴ时相卵母细胞和受精卵的卵细胞粘丝的外部形态特征和它们的粘性，并讨论了卵细胞粘丝的功能。     

支持细胞中促卵泡素信号通路研究进展

支持细胞在精子生成过程中起重要作用,支持细胞的数量决定睾丸大小、生精细胞数量以及最终生成精子数量。促卵泡素作为保证雄性生育能力的重要激素之一,通过与支持细胞上的促卵泡素受体结合,诱导5种信号途径,导致支持细胞中各类转录因子被激活,引起基因表达发生变化,从而保证生精细胞顺利发育成精子。文章主要围绕支持细胞中促卵泡素信号途径,及其对细胞发育过程中相关基因表达的影响等方面进行了综述。     

红叶石楠离体培养技术研究

以红叶石楠半木质化带芽茎段为外植体,探讨不同外源激素水平对其不定芽分化、增殖与不定根形成的影响。结果表明:MS BA 1.0~2.0 mg/L IBA 0.1~0.3 mg/L GA 0.5 mg/L的分化增殖效果好;增殖系数达6.5以上;White NAA0.1 mg/L AC(活性炭)0.5%或White IBA 0.1 mg/L AC 0.5%或White IAA 0.5 mg/L AC 0.5%的生根效果较好,生根率可达90.5%以上;在珍珠岩∶蛭石∶腐叶土=5∶2∶1的基质中炼苗,成活率可达96%以上。     

软枣猕猴桃‘奇异莓6号’离体再生技术

以软枣猕猴桃无芽茎段为外植体进行离体培养,具有成本低、取材方便、材料充足等优点,但以往的研究表明无芽茎段诱导再生率低。本试验以‘奇异莓6号’软枣猕猴桃无芽茎段为外植体,探究不同植物生长调节剂、光照强度、温度、苗龄对不定芽诱导的影响。结果表明：最佳外植体为苗龄30d的无芽茎段,在光照12h/d(光照强度50LX)、室温20℃下,不定芽诱导的最适培养基为MS+2mg/L ZT,不定芽以间接途径发生,培养40d无芽茎段两端开始形成淡绿色愈伤组织,培养45d愈伤组织表面出现红色小点,开始形成不定芽,培养55d愈伤组织诱导率、愈伤组织分化率及不定芽数均到最大,分别为100%、100%及18.87个/块。待苗长至3cm左右时转到MS+0.4mg/L ^IBA中进行生根培养,培养30d生根率可达100%、根数为8.53/株、根长1.68cm、根粗0.14cm。     

辣木的染色体制片优化及核型分析

以辣木分生组织为材料,采用酶解去壁低渗法制片,探讨不同取材部位、预处理方式和酶解时间对辣木染色体制片的影响,并对其进行核型分析,以期为辣木的起源、演化及遗传育种提供一定理论依据。结果表明:以辣木新枝茎尖为最佳取材部位,用饱和对二氯苯预处理2 h,再用4%纤维素酶和5%果胶酶混合物酶解4 h,制片所得染色体效果最佳。核型分析表明,辣木染色体属于小染色体,有28条,核型公式为2n=2x=2n=28m,属于1B类型,核型不对称系数60.29%,核型对称程度较高,这表明辣木在进化中可能处于比较原始类型。     

Mouse melanoma cell exosomes promote expression of Rac1 protein in fibroblasts

AIM To investigate the effect of exosomes secreted by mouse melanoma cells on the expression of Ras-related C3 botulinum toxin substrate 1 (Rac1) protein in fibroblasts. METHODS Ultracentrifugation was adopted to separete exosomes secreted by mouse melanoma B16-F10 cells. The morphological structure of exosomes was observed by negative-staining electron microscopy. The size distribution of exosomes was determined by nanoparticle tracking analysis (NTA). The exosomal markers, tumor susceptibility gene 101 (Tsg101) and tyrosinase-related protein 2 (Tyrp2), were identified by Western blot. Laser confocal microscopy was used to observe the process that mouse embryonic fibroblasts (MEF) took in exosomes during co-culture. Immunocytochemical staining and Western blot were used to detect the expression of Rac1 protein in MEF. RESULTS B16-F10 cell exosomes showed a typical tea tray-like structure, with a size range of 141~255 nm, and expressed protein markers Tsg101 and Tyrp2. The results of laser confocal microscopy showed that compared with co-culture at 0 h, a small number of exosomes appeared in the MEF at 12 h, and a large number of exosomes accumulated in the MEF after co-cultured for 24 and 36 h. Western blot analysis showed that compared with co-culture at 0 h, the expression of Rac1 protein in the MEF was significantly increased at 24 h and 36 h of co-culture (P<0.01). The results of immunocytochemical staining showed that compared with co-culture at 0 h, the positive expression level of Rac1 in the MEF cells was significantly increased at 12 h, 24 h and 36 h of co-culture (P<0.05 or P<0.01). CONCLUSION Intake of exosomes secreted by mouse melanoma cells promotes the expression of Rac1 protein in fibroblasts.     

Effects of different active constituents of Gynostemma pentaphyllum on mitochondrial energy metabolism-related proteins in endothelial cells induced by ox-LDL

AIM To investigate the effects of different components of Gynostemma pentaphyllum ［gypenosides (Gps), gypenoside XLIX (GpXLIX) and ginsenoside Rb3 (GRb3)］ on mitochondrial energy metabolism-related proteins in endothelial cells induced by oxidized low-density lipoprotein (ox-LDL). METHODS EA.hy926 cells were divided into control group, model group, Gps group, GpXLIX group and GRb3 group. The cells in control group were cultured only in DMEM complete medium. The cells in model group were treated with 100 mg/L ox-LDL for 48 h. The cells in Gps group, GpXLIX group and GRb3 group were treated with 100 mg/L ox-LDL for 24 h, and then treated with Gps, GpXLIX and GRb3 at 100 mg/L for another 24 h, respectively. The ATP content in each group was detected by ELISA. The expression levels of mitochondrial energy metabolism-related proteins, cytochrome C oxidase subunit 5a （Cox5a）, NADH:ubiquinone oxidoreductase core subunit S1 （Ndufs1）, ATP synthase F1 subunit alpha (ATP5a) and cytochrome C (Cyt C）, were determined by Wes automatic Western blot quantitative analysis system and Western blot. RESULTS Compared with control group, the ATP content in model group was decreased (P<0.01). After drug intervention, the ATP content increased to different degrees in Gps group, GpXLIX group and GRb3 group (P<0.01). The results of Wes automatic Western blot quantitative analysis system were consistent with those of Western blot. These results showed that compared with control group, the protein expression of Cox5a, Ndufs1 and ATP5a in model group was decreased, and the protein expression of Cyt C was increased (P<0.01). After intervention, the protein expression of Cox5a, Ndufs1 and ATP5a was increased and the protein expression of Cyt C was decreased in Gps group, GpXLIX group and GRb3 group (P<0.05 or P<0.01). Among them, the effect of Gps on the protein expression of Cox5a, Ndufs1 and Cyt C was significantly stronger than those of the 2 monomer components, and the effect of GRb3 was found to be superior in the 2 monomer components. The effect of GpXLIX on ATP5a protein was superior to the other 2 components. CONCLUSION Gynostemma total saponins and related active ingredients protect ox-LDL-induced endothelial cells by affecting mitochondrial energy metabolism-related proteins, thereby preventing and treating atherosclerosis.