Down-regulation of miR-153-3p attenuates H2O2-induced H9C2 cell injury by promoting Nrf2 expression

AIM To study the effect of microRNA-153-3p (miR-153-3p) knock-down on oxidative injury of H9C2 cells induced by H₂O₂ and its specific mechanism. METHODS The oxidative stress injury of H9C2 cell model was induced by H₂O₂, and then the cell viability and the expression of miR-153-3p were detected by MTT assay and RT-qPCR, respectively. The effects of miR-153-3p knock-down on the H9C2 cell injury under oxidative stress were studied by RNA interference technology. The targets of miR-153-3p were identified by Western blot and dual-luciferase reporter assay. RESULTS MTT assay showed that the viability of H9C2 cells was decreased with the increase in H₂O₂ concentration (P<0.05). The results of RT-qPCR showed that the expression of miR-153-3p was increased with the increase in H₂O₂ concentration (P<0.05). Knock-down of miR-153-3p increased the viability of H9C2 cells under oxidative stress, decreased the cell apoptosis and the content of malondialdehyde (MDA), and increased the activity of superoxide dismutase (SOD). The expression of nuclear factor E2-related factor 2（Nrf2） and antioxidant response element（ARE） activity were increased with the increase in H₂O₂ concentration (P<0.01). TargetScan analysis and dual-luciferase reporter assay showed that Nrf2 was one of the potential target genes of miR-153-3p. The results of Western blot further showed that over-expression of miR-153-3p inhibited the expression of Nrf2 (P<0.01), while down-regulation of miR-153-3p increased the expression of Nrf2 (P<0.01). Dual interference with Nrf2 and miR-153-3p significantly reduced H9C2 cell viability， promoted the apoptosis, increased MDA content, and decreased SOD activity in the presence of H₂O₂ (P<0.01). CONCLUSION Inhibition of miR-153-3p expression attenuates the injury of H9C2 cells induced by H₂O₂ through up-regulating Nrf2/ARE signaling pathway.     

芜菁Br14-3-3的克隆及其在非生物胁迫下的表达分析

克隆了‘津田芜菁’（Brassica rapa subsp. rapifera‘Tsuda’）通用调节因子14-3-3基因cDNA序列，命名为Br14-3-3（GenBank登录号为MK896872）。该基因全长1 113 bp，开放阅读框全长774 bp，编码含有257个氨基酸的多肽。荧光定量PCR分析Br14-3-3在‘津田芜菁’不同组织中及其在温度、脱水、渗透、ABA和无机盐等非生物胁迫下幼苗中的表达，结果表明该基因在‘津田芜菁’的花中表达量最高，幼苗中次之；低温抑制了Br14-3-3的表达，其他非生物胁迫可诱导该基因表达，暗示Br14-3-3在非生物胁迫应答中发挥功能。     

不同营养水平日粮对陕北白绒山羊生长性能和小肠组织SLC7A7、SLC3A1及SLC15A1 mRNA表达的影响

本试验旨在研究日粮营养水平对断奶后2~6月龄陕北白绒山羊生长性能及小肠组织中与氨基酸转运吸收相关的SLC7A7、SLC3A1和SLC15A1 mRNA表达的影响。选取健康、日龄（（60±1.60）d）和体重（（10.73±1.03）kg）相近的雌性陕北白绒山羊羔羊36只，随机分为4组，分别饲喂4种试验日粮，其消化能和粗蛋白质水平分别为标准日粮的85%、100%、115%和130%。标准日粮营养水平参考肉羊饲养标准NY/T816-2004，依据生长阶段（10~19 kg、15~27 kg）和目标增重设置。试验期间，分别于120和180日龄称重，于180日龄，每个重复屠宰1只试验羊，采集十二指肠中上部、空肠中段、回肠末端组织样品，通过实时荧光定量PCR检测SLC7A7、SLC3A1和SLC15A1表达水平。结果表明：1）第一阶段（60~120 d）115%水平组平均日增重显著高于其他三组（P<0.05），第二阶段（121~180 d）115%水平组平均日增重显著高于85%和100%水平组（P<0.05），与130%水平组无明显差异。两阶段115%水平组羔羊干物质采食量极显著高于其他3组（P<0.01）。两阶段料重比115%水平组显著低于85%、100%水平组（P<0.05）。2）相同营养水平下，SLC7A7和SLC15A1 mRNA的表达丰度顺序均为回肠>空肠>十二指肠；3）随日粮营养水平的增加，SLC7A7、SLC3A1和SLC15A1 mRNA在小肠各段的相对表达量呈先上升后下降的趋势，且115%水平组表达量最高。115%水平组SLC7A7和SLC15A1 mRNA相对表达量显著高于其他3组（P<0.05）；115%水平组SLC3A1 mRNA的相对表达量显著高于85%和130%水平组组（P<0.05）。本试验条件下，与其他营养水平组相比，115%水平组陕北白绒山羊羔羊在2~6月龄生长性能最佳，SLC7A7、SLC3A1和SLC15A1 mRNA在小肠各段的表达量最高。     

Effects of DHRS3 in C2C12 Myoblast Differentiation and Mouse Skeletal Muscle Injury

Myoblast differentiation is an essential process during skeletal muscle development. C2 C12 myoblast is a commonly used experimental model to study muscle cell differentiation in vitro. Dehydrogenase/reductase(SDR family) member 3(DHRS3) is a highly conserved member in short-chain alcohol dehydrogenase/reductase superfamily and has been shown to be involved in the metabolism of retinol. Previous experimental results showed that the expression of DHRS3 increased significantly during the differentiation of myoblasts differentiation. However, the effect of DHRS3 on mouse muscle cell differentiation was unclear. The objective of current study was to determine if DHRS3 affected muscle cell differentiation, and if DHRS3 was involved in muscle regeneration. Protein expression was determined by western blot and immunofluorescence analysis. The activation and inhibition of DHRS3 increased and decreased C2 C12 myoblast differentiation respectively, which indicated that DHRS3 could affect C2 C12 myoblast differentiation. DHRS3 expression was significantly changed during muscle regeneration, with the regeneration of muscle injury, the expression of DHRS3 tended to increase first and then decrease. It suggested that DHRS3 might be involved in muscle regeneration. In summary, this study confirmed the involvement of DHRS3 in C2 C12 myoblast differentiation and mouse skeletal muscle regeneration and provided a theoretical basis for further elucidating the molecular mechanism of muscle development.     

光响应性阳离子表面活性剂PCDA-C6-NH3+的合成及其对液滴蒸发行为的调控

农药的有效利用与农药液滴在植物叶片上的蒸发过程息息相关。传统表面活性剂虽然可以改变液滴的蒸发模式或速率,但并不能根据外界环境变化对蒸发过程进行主动调节。为实现"自主调控"农药液滴蒸发的目的,本文设计合成了一种含丁二炔官能团的光响应性阳离子表面活性剂(PCDA-C6-NH3+),利用紫外光刺激改变其在液滴中的聚集状态,调控液滴的蒸发过程。该表面活性剂以10,12-二十五碳二炔酸(PCDA)作为骨架,通过酰胺化反应引入末端氨基并质子化后得到。采用紫外-可见光谱研究了PCDA-C6-NH3+的拓扑化学聚合反应,并利用静态表面张力和动态接触角分析了其紫外光照前后的表面活性和蒸发行为。该研究为实现液滴"自主调控"蒸发过程提供了一种新思路,对提高农药利用率具有重要意义。     

云南、广西三七黑斑病病原链格孢菌的鉴定

正黑斑病是三七栽培生产中常见的一大病害,叶片受害产生近圆形或不规则水浸状病斑,常导致成株落叶、幼苗生长点及茎秆顶端腐烂枯死。其病原一般认为是链格孢属真菌人参链格Alternaria panax Whetzel~([1,2]),也有相关研究证明黑斑病病原为细链格孢Alternaria tenuis Nees~([3]),后定名为链格孢Alternaria alternata Keissl~([4])。本研究利用ITS序列和histone 3部分编码序列的PCR鉴定,结合形态学鉴定,分析三七主产区黑斑病菌的组成和分布情况及几种病原菌的致病力差异,以期为三七黑斑病防治提供理论依据。     

Effects of antimicrobial peptides on growth,morphology of foregut villi and related genes mRNA expression in the common carp (Cyprinus carpio)

A 60‐day feeding trial was conducted to examine the effects of different levels (0, 100, 200, 400 and 600 mg/kg) of antimicrobial peptides on growth, protease activity of foregut, the morphology of foregut villi and related genes mRNA expression level in the common carp (Cyprinus carpio). The results showed that the feed of antimicrobial peptides promote common carp growth, and the optimal dosage of antimicrobial peptides is 200–333 mg/kg in the common carp feed. The protease activity of 200 and 400 mg/kg groups were significantly higher than the control and other groups (p < 0.05). The foregut villus height with 100, 200 and 400 mg/kg antimicrobial peptide groups were significantly higher than control group (p < 0.05). The crypt depth of 200 and 400 mg/kg antimicrobial peptide groups were significantly lower than control group (p < 0.05). The ratio of villus height and crypt depth of 100, 200 and 400 mg/kg antimicrobial peptide groups were significantly higher than control group (p < 0.05). The ratio with 600 mg/kg group was significantly lower than the control group (p < 0.05). The IGF‐I gene expression level of 200 mg/kg and 400 mg/kg groups were significantly higher than the control group and 600 mg/kg group (p < 0.05). The IL‐1β gene expression level of 100 mg/kg and 200 mg/kg groups were significantly higher than the control group (p < 0.05). These results indicated up‐regulation of growth and immune related genes in antimicrobial peptides fed common carp. Correlation analysis showed that IGF‐I mRNA and IL‐1β mRNA were positively correlated with SGR. IL‐1β mRNA and FCR were significantly negative correlated. It indicated that growth and immune gene common regulated the growth of the carp under antimicrobial peptides intervention. In conclusion, antimicrobial peptides can improve growth and related genes mRNA expression in the common carp. Further studies using molecular biological technique or immunologic methods are required to conclude that antimicrobial peptides are beneficial in common carp.