Role of ghrelin in cell protection by up-regulating HSP70 through ERK1/2 signaling pathway in PC12 cells

AIM:To study the role of ghrelin in cell protection by up-regulating heat shock protein 70 (HSP70) and inhibiting apoptosis induced by oxidative stress through extracellular regulated protein kinases 1/2 (ERK1/2) signaling pathway in the PC12 cells. METHODS:Sodium nitoprusside (SNP) was used to induce oxidative stress injury in the PC12 cells. The cultured PC12 cells were divided into SNP-injured group (incubated with SNP at 0.5 mmol/L for 6, 12, 18 and 24 h), ghrelin pretreatment group (ghrelin at 100 nmol/L was given 30 min before adding SNP); HSP70 inhibitor group (quercetin at 10 μmol/L was added 60 min before ghrelin treatment), ERK inhibitor group (ERK 1/2 inhibitor PD98059 was added 60 min before ghrelin treatment) and control group (added same amount of culture medium only). The apoptotic rate was detected by flow cytometry. The protein expression was determined by Western blot and immunocytochemistry. RESULTS:Compared with control group, the apoptotic rate of PC12 cells in SNP-injured group was significantly increased (P<0.05). Compared with SNP-injured group, ghrelin (100 nmol/L) pretreatment significantly inhibited SNP-induced apoptosis of PC12 cells (P<0.05), and significantly up-regulated the protein expression of HSP70 (P<0.05). Time-effect analysis showed that ghrelin had the most significant effect at 18 h after SNP injury. Quercetin, an inhibitor of HSP 70, significantly reduced the anti-apoptotic effect of ghrelin (P<0.05). Ghrelin pretreatment promoted the phosphorylation of ERK1/2. ERK1/2 inhibitor PD98059 significantly inhibited the effects of ghrelin on up-regulation of HSP70 expression (P<0.05). CONCLUSION:Ghrelin upregulates the expression of HSP70 and inhibits the apoptosis in the PC12 cells induced by oxidative stress by promoting the phosphorylation of ERK1/2.     

玉米热激蛋白ZmHSP70-12基因的克隆及表达分析

热激蛋白70(HSP70)是原核和真核细胞中普遍存在的一种高度保守的分子伴侣。从玉米中克隆1个HSP70家族成员。该基因cDNA序列全长为1 992 bp,开放阅读框为2 352 bp,编码663个氨基酸,蛋白质分子量约75.0 kD。蛋白结构预测及同源比对分析表明,该基因编码蛋白含ATPase位点和HSP70保守结构域,与拟南芥AtHSP70-12序列高度相似,命名为ZmHSP70-12。蛋白亚细胞定位显示,ZmHSP70-12蛋白在内质网中表达。实时荧光定量PCR分析表明,ZmHSP70-12对非生物胁迫高温、干旱均具有明显的应答反应,推测ZmHSP70-12是玉米中与胁迫逆境相关的基因。     

PVX病毒载体介导2种马铃薯Y病毒科病毒VPg蛋白表达诱导烟草叶片系统坏死的研究

芜菁花叶病毒（Turnip mosaic virus, TuMV）和槟榔坏死环斑病毒（Areca plam necrotic ringspot virus, ANRSV）是马铃薯Y病毒科（Potyviridae）中分别可诱导十字花科作物和槟榔产生坏死病症的2种不同属病毒。VPg（Viral protein genome linked）作为与马铃薯Y病毒科病毒基因组5′端的结合蛋白,在病毒复制、翻译和运动等侵染过程中发挥重要作用。本研究利用In-Fusion克隆策略分别构建了可表达3′端融合Strep蛋白标签序列的ANRSV和TuMV VPg全长编码基因的马铃薯X病毒（Potato virus X, PVX）载体pPVX-VPg-AR和pPVX-VPg-Tu。通过农杆菌渗透注射接种本生烟（Nicotiana benthamiana）,利用RT-PCR、Strep蛋白标签亲和层析和Western blot等方法证明了PVX病毒载体能够介导VPg-AR和VPg-Tu蛋白在本生烟中系统表达,且发现这2种VPg蛋白的过量表达诱导本生烟叶片产生了不同程度的系统性坏死病症。进一步采用DAB和NBT染色,在产生坏死症状叶片中检测到大量活性氧（reactive oxygen species, ROS）的积累。因此,推测VPg可能是TuMV和ANRSV诱发植物病症产生的一个决定因子,为后续研究这2种病毒诱导症状形成机制奠定了基础。     

保障中俄东线天然气管道长期安全运行的若干技术思考

针对中俄东线天然气管道的实际服役状况,分析了土壤运动(冻胀与解冻沉降)对管道结构完整性的影响以及基于管体结构-土壤弹簧模型在确定管-土交互作用方面的局限性,即非线性、大应变与多轴加载评估的保守性、土壤本构模拟与真实状况的偏离,建议发展新型多模块耦合集成技术确定土壤运动产生的机械效应。明确了X80高强管线钢在服役条件下发生应变时效及其导致管线钢(尤其是焊缝区)材料韧性和止裂能力的降低,建议使用时效活化能与等效时效时间模拟、评估管线钢在漫长服役过程中发生应变时效的敏感性,并建立相应的理论基础。此外,详细分析3种常见的管道缺陷(机械损伤、腐蚀缺陷、裂纹)对管道完整性影响的评估技术现状。针对高压、大口径、高强钢天然气管道(特别是焊接金属与热影响区)在地质不稳定地区的材料韧性、裂纹扩展以及止裂能力开展实验与评价技术,建立精确的多物理场协同作用下的管道缺陷评估模型,是当前的国际性技术难题,这些问题的解决将有力保障中俄东线天然气管道以及相关油气管道的长期安全运行。     

Development of a method for live octopus (Octopus vulgaris) transportation for long distance at high densities

The development of new octopus‐based products with a growing economic value ensures the commercial interest of this species, making live octopus export an activity of great interest. The aim of this study was to develop a method for long‐distance transportation of live octopus at high densities. The system was composed by 220‐L tanks with cooling and aeration, where the animals were kept separated from each others. The water temperature was maintained at 10°C, after a decreasing of 1°C/hr. Live octopus transportation was tested for 48 hr at two densities: 50 kg/m³ and 100 kg/m³. During this period, water parameters were monitored. Stress response was evaluated through the analysis of haemolymph, muscle and brain tissues. No mortality was registered after 48 hr for both treatments. In all trials, water quality remained within the normal limits in both densities; there was, however, a significative increase of ammonia levels in the water. Ammonia, dopamine and Hsp70 levels were analysed in the beginning and at the end of the experiment for both densities; however, no significant differences were found among them. In general, this system seems to be a viable solution for live octopus 48‐hr transportation at a density of 100 kg/m³.     

Outer membrane protein A of Acinetobacter baumannii induces autophagy via Akt/mTOR/p70S6K signaling pathway in RAW264.7 cells

AIM:To analyze the effects of outer membrane protein A (OmpA) from Acinetobacter baumannii ATCC 19606 on the autophagy of RAW264.7 cells. METHODS:The RAW264.7 cell model stimulated by OmpA was established. The effects of OmpA on the autophagy of RAW264.7 cells were detected by immunofluorescence, Western blot and transmission electron microscopy. RESULTS:The OmpA increased the expression of LC3B-Ⅱ and reduced the phosphorylation levels of Akt, mTOR and p70S6K. Rapamycin further reduced the phosphorylation levels of mTOR and p-70S6K, and increased the expression of LC3B-Ⅱ induced by OmpA. CONCLUSION:The OmpA of Acinetobacter baumannii induces autophagy via Akt/mTOR/p70S6K signaling pathway in the RAW264.7 cells. This work provides a basis for further research on the molecular mechanism of autophagy induced by Acinetobacter baumannii to find a new method against the infection of Acinetobacter baumannii.     

中国杧果科学研究70年

新中国成立70年来,我国杧果科学研究在人才培养与团队建设、硬件平台、基础理论创新与技术研发等方面均取得了重要进展,有力支撑了我国杧果产业的创建和可持续发展。本文在概述世界和我国杧果地位、分布、规模的基础上,从科学研究发展历程、种质资源与遗传育种、土壤与肥水管理、耕作模式与花果管理、病虫害防控、采后贮运保鲜、产业经济等方面全面梳理了我国杧果研究取得的成就,分析了存在的不足并提出了未来的重点发展方向。     

文心兰HSP70基因的克隆及表达分析

为研究文心兰热激蛋白70基因（命名为OnHSP70）的分子特性及表达特点,以文心兰‘柠檬绿’（Oncidium hybridum ‘Honey Angel’）为材料,采用RT-PCR技术克隆OnHSP70,利用生物信息学方法分析其分子特性,通过qRT-PCR技术分析其在不同组织及不同非生物胁迫处理下的表达特点。生物信息学分析表明：该基因开放阅读框为1944 bp,编码647个氨基酸,翻译的蛋白为稳定蛋白,属于HSP70超家族,其蛋白二级结构由41.11%的α-螺旋、17.77%的延伸链、7.73%的β-转角和33.38%的无规卷曲组成,具有2个高度保守的功能域。聚类分析表明：该蛋白与铁皮石斛和深圳拟兰的HSP70亲缘关系较近。qRT-PCR分析表明：文心兰HSP70在4种不同组织器官中具有表达差异性,在花中的表达量最高;高温处理后基因的表达量明显上升;40 ℃高温胁迫4 h时表达量达峰值;茉莉酸甲酯及水杨酸处理时表达量呈现下调响应。本研究为后期该基因功能研究及提高文心兰对高温的适应性提供理论基础。     

木塑与钢材复合温室骨架设计及力学性能试验

木塑复合材料是近几年发展较快的一种新型材料,具有易加工、密度高、硬度强的特点。为探究木塑在温室建筑上的应用,设计了一种适合温室使用的木塑与钢材复合骨架,并进行力学性能试验。该试验以木塑和钢材为试材,采用拉伸、压缩、人工气候老化及复合骨架应用于温室的方法,研究了其抗拉、抗压强度及其在温室中应用情况,以期能够开发一种在性能和价格上与钢骨架结构材料相媲美的新材料。结果表明:在低温、室温和高温条件下,木塑的抗拉强度分别为28.391、24.954、15.000 MPa,木塑的抗压强度分别为63.633、42.438、32.547 MPa,木塑的抗拉强度和抗压强度均与环境温度呈负相关关系。木塑在经过250 h的人工气候老化后的抗弯强度为37.040 MPa,比未进行老化处理下降了22.083%。将木塑与钢材结合制作成不同形式的复合骨架,与普通木塑骨架对比,在室温下测试发现复合骨架比普通木塑骨架抗弯性能显著提高,其延展性提高约3倍,其中钢材添加在下缘的复合骨架的抗弯性能显著较钢材在上缘的复合骨架优越;带卡簧卡槽复合骨架的最大抗弯屈服力为19.112 kN,较钢材在下缘的复合骨架提高88.74%,达到了温室骨架的承载力要求。通过供试带卡簧卡槽复合骨架温室的荷载试验得出,跨度8.0 m、顶高3.3 m的拱形屋面温室,其骨架间距为1.2 m时,供试温室承受荷载为0.436 kN·m^-2;当骨架间距为1.0 m时,其承受荷载为0.527 kN·m^-2。与传统钢骨架温室对比,复合骨架温室的建筑成本减少了10.4元·m^-2。该复合骨架可以同时发挥木塑的环保、价廉、可塑性优势和钢材的优良力学性能,为温室建筑的轻简化、装配化提供了有益参考。     

烟草Hsc70-2的克隆及对马铃薯Y病毒侵染烟草的促进作用

【目的】马铃薯Y病毒（Potato virus Y,PVY）是危害烟草、马铃薯、番茄、辣椒等主要农作物的重要病毒,给农业生产带来巨大损失。论文旨在克隆Hsc70-2蛋白在本氏烟（Nicotiana benthamiana）中的基因序列并分析其生物学信息,研究NbHsc70-2蛋白对PVY侵染烟草的影响,为进一步解析PVY的侵染机制提供理论依据。【方法】以本氏烟为材料,克隆NbHsc70-2蛋白的基因编码序列（coding sequence,CDS）,利用MEGA 6.0 进行多序列比对并构建系统进化树;利用实时荧光定量PCR（qRT-PCR）分析NbHsc70-2在本氏烟各组织中的表达水平;采用在线软件BaCeILo和SignalP 4.0对NbHsc70-2进行生物信息学分析;构建NbHsc70-2-RFP融合蛋白确定该蛋白的亚细胞定位;研究PVY处理对本氏烟叶片中NbHsc70-2的影响;利用激光共聚焦观察PVY-GFP处理对NbHsc70-2-RFP定位的影响;构建NbHsc70-2 VIGS沉默体系及瞬时表达载体,采用qRT-PCR比较NbHsc70-2在沉默/过表达后对PVY表达的影响。【结果】NbHsc70-2编码649个氨基酸,系统进化树分析表明,NbHsc70-2与普通烟NaHsc70-2序列相似性最高,亲缘关系最近,属于热激蛋白家族,C端具有热激蛋白家族的高度保守基序结构;qRT-PCR分析表明,NbHsc70-2在叶中表达量最高,在根和茎中的表达量较低;BaCeILo预测及激光共聚焦显微镜观察均显示NbHsc70-2定位在细胞质中,并且PVY-GFP侵染本氏烟后NbHsc70-2-RFP部分转移至细胞核,与PVY-GFP共定位在细胞质及细胞核中;将NbHsc70-2基因沉默载体pTRV::NbHsc70-2导入本氏烟中7 d后相比于对照组,沉默组出现心叶皱缩及矮化现象;接种PVY-GFP 7 d后通过手持紫外灯观察到沉默组中无明显绿色荧光出现,而对照组中PVY-GFP系统侵染使得非接种叶片呈现荧光现象,沉默组荧光点数约为对照组28%;接种PVY后,利用qRT-PCR检测沉默NbHsc70-2后1、3、5 d的PVY CP基因积累量,结果表明沉默NbHsc70-2后PVY CP基因积累量下降,其中3 d和5 d与对照相比差异显著,基因表达水平分别为对照的14%和0.004%;将NbHsc70-2过表达载体pEarleyGate100::GWC::NbHsc70-2与PVY同时导入本氏烟后,结果表明相比于对照组,过表达组48 h和72 h 其PVY CP基因积累量显著上升,基因表达水平分别为对照组的2.31、2.56倍。【结论】PVY侵染会引起NbHsc70-2表达量上升;NbHsc70-2是PVY侵染本氏烟重要的组成成分,沉默该基因显著抑制PVY的表达,过表达NbHsc70-2则显著提高PVY的表达,即NbHsc70-2的表达水平与PVY复制呈正相关,NbHsc70-2蛋白促进PVY对烟草的侵染。