XBP-1u suppresses autophagy by promoting the degradation of FoxO1 in cancer cells

Autophagy is activated to maintain cellular energy homeostasis in response to nutrient starvation. However, autophagy is not persistently activated, which is poorly understood at a mechanistic level. Here, we report that turnover of FoxO1 is involved in the dynamic autophagic process caused by glutamine starvation. X-box-binding protein-1u (XBP-1u) has a critical role in FoxO1 degradation by recruiting FoxO1 to the 20S proteasome. In addition, the phosphorylation of XBP-1u by extracellular regulated protein kinases1/2 (ERK1/2) on Ser61 and Ser176 was found to be critical for the increased interaction between XBP-1u and FoxO1 upon glutamine starvation. Furthermore, knockdown of XBP-1u caused the sustained level of FoxO1 and the persistent activation of autophagy, leading to a significant decrease in cell viability. Finally, the inverse correlation between XBP-1u and FoxO1 expression agrees well with the expression profiles observed in many human cancer tissues. Thus, our findings link the dynamic process of autophagy to XBP-1u-induced FoxO1 degradation.     

单纯疱疹病毒1型引起的发热出疹性疾病需要与手足口病进行鉴别

对2008年在甘肃省发生的一起疑似手足口病(HFMD)的发热出疹性疾病的流行进行病原体的实验室检测,明确引起这起传染病流行的病原体。从4名发热出疹患者采集的8份临床标本中(每个患者采集咽拭子和疱疹液标本),首先将临床标本接种到RD和HEp-2细胞上进行病毒分离,对病毒分离阳性的标本提取病毒核酸,然后使用荧光定量-逆转录-聚合酶链式反应(RT-PCR)进行人肠道病毒(HEV)核酸的检测。对HEV检测结果阴性的标本采用序列非依赖的单引物扩增技术(SISPA)进行"未知病原体"的鉴定。分离到的6株病毒均鉴定为单纯疱疹病毒I型(HSV-1),结合分析这起流行中患者的临床表现、流行病学调查结果以及实验室检测结果,表明HSV-1是引起这起发热出疹性疾病流行的病原体。6株HSV-1的gG区核苷酸和氨基酸水平上差异都较小,同源性分别高达98.8%和97.9%,说明这起疫情是由同一个病毒传播链引起的。HSV-1等病毒引起的发热出疹性疾病需要与HFMD进行鉴别诊断,由于仅从临床症状和流行病学资料上判断引起发热出疹性疾病的病原体是非常困难的,因此,必须依赖于实验室的诊断。     

ERK介导的炎性反应参与肾缺血再灌注损伤

目的研究小鼠肾缺血再灌注损伤的发病机制。方法建立小鼠肾缺血再灌注损伤模型。12只雄性C57BL／6随机分为2个组（n=6）,分别为假手术组（Sham）,肾缺血再灌注损伤模型组（IRI）。IRI组血管夹夹闭左肾动脉,置于32℃温箱后1h松开血管夹,去除右肾。Sham组操作同上,但不夹闭左肾动脉。再灌注24h后处死小鼠,收集血清和肾脏标本。测定血清肌酐（Cr）和血尿素氮（BUN）。PAS染色后显微镜下观察肾脏形态学变化,Western印迹分析ERK、p-ERK的表达,PCR检测MCP-1、IFN-γ。结果与假手术组（Sham）相比,IRI组血清肌酐、血尿素氮明显升高,病理检查可见肾脏内肾小管上皮细胞明显肿胀坏死、蛋白管型形成明显,还可观察到炎性细胞浸润明显增加。ERK、p-ERKWestern印迹结果PCR显示MCP-1、TNF-α也明显上调,但ERK表达不变。结论在肾缺血再灌注中,ERK激活介导的炎性后府可能参与了肾扣伤。     

石参总黄酮对一氧化氮致大鼠胰岛细胞损伤的保护作用

采用硝普钠为NO供体,造成大鼠胰岛β细胞RIN-m的损伤,通过检测细胞活力、细胞内丙二醛(MAD)含量、总谷胱甘肽(GSH)含量和总超氧化物歧化酶(SOD)活性,探讨石参总黄酮的保护作用和机制。结果显示,石参总黄酮能明显提高损伤细胞的活力,降低细胞内MDA的含量、提高总GSH含量和SOD活力,表明石参总黄酮对NO所致RIN-m细胞的损伤具有保护作用,其机制可能与提高细胞内GSH含量与SOD活力有关。     

独脚金内酯调控植物侧枝发育的分子机制及其与生长素交互作用的研究进展

对独脚金内酯（strigolactones,SLs）调控植物侧枝发育的分子机制及其与生长素相互作用的相关研究结果进行了总结和归纳,在此基础上提出今后的重点研究方向。相关的研究结果显示：在拟南芥[Arabidops~thaliana（Linn．）Heynh．]、豌豆（Pisum sativum Linn．）和水稻（Oryza sativa Linn．）等植物多枝突变体中SLs作为可转导信号参与侧枝发育的分子调控,从这些植物中已克隆获得参与SLs生物合成及信号应答途径的一些基因。作为一种植物激素,SLs在侧枝发育调控网络中与生长素相互作用;腋芽发育与其中生长素的输出密切相关,SLs通过调控芽中生长素的输出间接抑制腋芽发育和侧枝生长,而生长素则在SLs生物合成中起调节作用。     

土壤干旱胁迫对九头狮子草和圆苞金足草幼苗形态和生理特性的影响

采用称重控水法控制土壤相对含水量分别为(85.0±2.5)％(对照)、(67.5±2.5)％(轻度干旱)、(50.0±2.5)％(中度干旱)和(32.5±2.5)％(重度干旱),对土壤干旱胁迫条件下九头狮子草[Peristrophe japonica (Thunb.)Bremek.]和圆苞金足草(Goldfussia pentstemonoides Nees)2年生苗的植株形态及生理特性变化进行了研究.结果表明:经土壤干旱胁迫处理30 d后供试2种植物的外部形态均有一定变化,其中九头狮子草主要变化为叶片失绿、变薄且萎蔫、枝条下垂;圆苞金足草主要变化为茎干倒伏、叶片变软且叶柄低垂.随土壤干旱胁迫程度的增加,供试2种植物叶片的自然饱和亏、临界饱和亏、需水程度、束缚水含量、束缚水与自由水的含量比值、脯氨酸含量和可溶性糖含量均呈逐渐增加的趋势且均高于对照,而自由水含量、最高水势、最低水势和可溶性蛋白质含量均逐渐降低且总体上低于对照.总体上看,在重度干旱胁迫条件下供试2种植物各生理特性均与对照有极显著或显著差异,而在轻度或中度干旱胁迫条件下部分指标与对照无显著差异.供试2种植物各生理指标的变化幅度有明显差异,在同一干旱胁迫条件下九头狮子草叶片的自然饱和亏、需水程度、自由水含量、最高水势和最低水势的降幅、脯氨酸含量和可溶性蛋白质含量的降幅均高于圆苞金足草,其临界饱和亏、束缚水含量、束缚水与自由水的含量比值和可溶性糖含量均低于圆苞金足草.综合分析结果表明:供试2种植物对土壤干旱胁迫均具有一定的耐性,但圆苞金足草具有更强的抵御干旱的生理机制.     

N—acetylserotonin对肝缺血再灌注小鼠氧化应激损伤的保护作用

目的探讨NAS对肝缺血再灌注所诱导的脂质过氧化损伤产生的保护作用。方法采用夹闭肝蒂法30min、再灌注6h制作肝缺血再灌注模型,冰冻切片,HE染色,光学显微镜下观察肝细胞形态结构的变化;比色法检测损伤后血清中谷丙转氨酶（ALT）水平及肝组织中超氧化物歧化酶（SOD）、丙二醛（MDA）、谷胱甘肽过氧化物酶（GSH—Px）的含量。结果夹闭肝蒂30min、再灌注6h后,肝小叶结构紊乱、肝血窦淤血,其间有白细胞浸润、肝细胞出现变性、坏死;血清中ALT水平升高,肝组织中s0D和GSH—Px的含量降低,MDA升高;NAS可减少缺血再灌注后血清ALT的释放,使肝组织中SOD和GSHPx的含量升高,MDA的含量降低;NAS＋Luz可逆转NAS的这一作用。结论NAS对肝缺血再灌注小鼠的氧化应激损伤具有保护作用。     

Screening tomato-associated bacteria for biological control of grey mold on tomato

Aiming at discovering effective biocontrol agents (BCAs) against grey mold on tomato caused by Botrytis cinerea Pers., we selected 819 bacterial isolates from the surface as well as the interior of the roots, stems, and leaves of tomato plants grown in B. cinerea-infested fields. In a dual-culture assay, 116 isolates (14.16%) showed antagonism against B. cinerea and fewer ones against five additional tomato-associated fungal pathogens – Pythium ultimum, Phytophthora capsici, Fusarium oxysporum f. sp. lycopersici, Sclerotinia sclerotiorum and Ralstonia solanacearum. Thirty-one isolates with antagonism to B. cinerea and at least one of the five additional pathogens were assessed for their efficacy in controlling grey mold on tomato in a greenhouse test. Thirteen of them attained the efficacy over 50% and were subjected to the second greenhouse test, in which 12 isolates consistently accomplished the biocontrol efficacy over 50%, with isolates ABc28 and ABc22 achieving the efficacy of 66.71% and 64.90%, respectively. Under greenhouse conditions, the above two as well as isolates ABc2, ABc11 and ABc17 increased tomato biomass by more than 20% in comparison with the control. The 12 antagonistic isolates accomplishing the biocontrol efficacy over 50% in both greenhouse tests were considered potential BCAs against grey mold, which were identified as Pseudomonas spp., Pantoea spp., Bacillus spp. and Chryseobacterium spp. Ten of them were found to produce at least one of the three hydrolytic enzymes (protease, cellulase and chitinase) and/or siderophore, which might be involved in their mechanisms of suppressing the disease. Based on the origin of these 12 strains, the leaf tissue, especially the leaf interior, of tomato plants grown in a B. cinerea-infested field appears to be a good source of potential BCAs against grey mold.