重组GSTA3蛋白对福美双诱导的肉鸡TD中抗凋亡基因BAG-3表达的影响

【目的】肉鸡胫骨软骨发育不良（TD）是肉鸡常见的一种骨骼性疾病,研究重组GSTA3蛋白对福美双诱导的TD肉鸡软骨细胞中抗凋亡基因BAG-3表达的影响,为治疗TD提供新的思路和方法。【方法】将120羽1周龄肉雏鸡随机分为6组（编号为A、B、C、D、E、F组）。A、B、C组为基础日粮对照组,D、E、F组为添加福美双日粮诱导TD组。试验饲喂福美双2 d诱发TD,在添加福美双第1、3、5、7天,腿部肌肉注射重组鸡GSTA3蛋白和磷酸盐缓冲液,A组与D组注射（100 μg·kg ^-1）磷酸盐缓冲液;B组与E组注射低剂量（100 μg·kg ^-1）GSTA3;C组与F组注射高剂量（200 μg·kg ^-1）GSTA3。试验历时23 d。添加福美双后1、2、4、6、10和15 d采集胫骨生长板。通过Real-time qPCR检测BAG-3基因的mRNA水平,利用免疫组化来检测BAG-3蛋白表达水平。【结果】Real-time qPCR结果显示,TD损伤修复期内,相比较于基础日粮对照组,福美双对照组肉鸡胫骨生长板中BAG-3 mRNA的表达水平基本都显著上调（P<0.05）;相比较于福美双对照组,E和F组在第2、4、10、15天都有显著差异,且在第10和15天显著低于福美双对照组（P<0.05）,表明与D组相比恢复较快。免疫组化结果表明BAG-3蛋白在肉鸡胫骨软骨细胞的增殖区和前肥大区无表达,只在肥大区细胞质中表达;福美双组与空白对照组相比,BAG-3蛋白表达增加;福美双高低剂量组与未注射蛋白的福美双组相比,重组GSTA3增加了肥大区的蛋白表达水平（第10和15天）。【结论】在福美双诱导肉鸡发生TD的过程中,GSTA3重组蛋白能够通过调控BAG-3表达参与凋亡途径,抑制细胞凋亡。在TD损伤修复期,注射GSTA3后使抗凋亡基因BAG-3蛋白表达增强,从而可参与细胞凋亡来缓解TD损伤,使得肉鸡TD生长板功能较快地恢复正常。     

基于转录组测序开发糜子SSR标记

【目的】 以6份不同地理来源的糜子资源为试验材料,基于前期转录组测序获得的1 000对SSR引物,选出200对进行多态性检测,以期构建一批可以准确评估糜子种质遗传差异的分子标记。【方法】 用Primer Premier 5.0软件设计引物,改良CTAB法提取DNA,PCR扩增DNA和聚丙烯酰胺凝胶电泳筛选引物多态性;用PowerMarker 3.25和PopGen 1.32计算遗传多样性参数。【结果】 200对引物中97对呈单态性,80对呈多态性。单碱基序列重复引物有20对,10对具多态性,其重复基元是A（50%）和T（50%）。二碱基序列重复引物有36对,15对具多态性,其碱基重复类型有7种（AG最多,TC、GC和GA次之,CA、TA和AC最少）。三碱基序列重复引物有144对,55对具多态性,其碱基重复类型有24种（GGC、GCG和GCC最多,GAA、GCT和CGC等次之,ACC、AGG、CAG、CGT、AAG、AAC、TCG、CGA、ATT、CAA和CCA最少）。就引物分辨率(Rp)值而言,1—3碱基序列重复引物分别为0.67—4.67（平均2.07）、1.33—4.33（平均2.73）和0.67—4.00（平均1.83）。基于Rp值分析SSR分布频次,发现80个标记分布在5个区间：0—1、1—2、2—3、3—4和4—5,分别包含17（21.25%）、36（45.00%）、11（13.75%）、14（17.50%）和2个（2.50%）。就$\overline{\text{Rp}}$值而言,1—3碱基序列重复引物分别为0.33—0.67（平均0.51）、0.40—0.78（平均0.59）和0.33—0.83（平均0.59）。单碱基序列重复标记共检测到22个等位变异,每个位点为2—3个（平均2.2000）,其中8个和2个位点分别具2和3个变异;二碱基序列重复标记共检测到38个等位变异,每个位点为2—3个（平均2.5333）,其中7个和8个位点分别具2和3个变异;三碱基重复标记共检测到136个等位变异,每个位点为2—3个（平均2.4727）,其中29个和26个位点分别具2和3个变异。就多态性信息含量而言,1—3碱基序列重复引物分别为0.3750—0.5355（平均0.4293）、0.2392—0.7438（平均0.4293）和0.2392—0.7438（平均0.3989）。就多样性指数而言,1—3碱基序列重复分别为0.6365—1.0776（平均0.7497）、0.5623—1.0986（平均0.8339）和0.5623—1.0889（平均0.8312）。【结论】 基于转录组测序结果,检测200对SSR引物的多态性,发现177对（88.5%）可以扩增出完整条带,其中80对具多态性,多态率为40%。     

土壤日晒在绿色植保中的应用与展望

土壤消毒主要用于土壤病虫草害防控。过去几十年,土壤主要采用化学药品熏蒸消毒,不合理使用容易造成环境污染。土壤蒸汽消毒、火焰消毒和热水浇灌等需要专门的仪器设备,且存在能耗较高、灭生性强、容易破坏土壤结构等缺点。目前,土壤日晒技术受到意大利、美国、以色列等70多个国家农业科学家的广泛关注,但在中国依然处于初级阶段。本文总结了国内外学者关于土壤日晒对农业病虫草害、土壤肥力、农作物产量等方面的影响与应用,分析了土壤日晒存在的局限性,并对土壤日晒在未来农业绿色防控上的应用前景进行了展望,以期为农产品无公害生产提供理论依据和实践参考。     

水稻温敏型叶片白化转绿突变体tsa2的表型鉴定与基因定位

水稻温敏型叶色突变体是研究植物光合作用、叶绿体结构和功能以及温度影响叶绿体发育的理想材料。利用甲基磺酸乙酯(EMS)诱变籼型水稻(OryzasativaL.)三系保持系西农1B,从其后代中筛选到一个突变性状稳定遗传的温敏型叶片白化转绿突变体tsa2 (temperature-sensitive green-revertible albino 2)。与野生型相比, tsa2突变表型受温度影响, 22°C条件下萌发的野生型幼苗表型正常,而tsa2幼苗完全白化,且约40%白化苗死亡,存活白化苗的光合色素含量、光合速率均显著降低,成熟期主要农艺性状均显著变劣;在28°C下萌发的tsa2幼苗叶片呈浅绿色并伴有白条纹,其光合色素含量显著降低,光合速率及主要农艺性状差异较小; 32°C下萌发的tsa2幼苗叶片无明显差异。透射电镜观察显示,与野生型相比,tsa2在22°C下叶肉细胞中无叶绿体或存在异常发育叶绿体(尚未分化出基粒和基层),在28°C下部分叶肉细胞含少量发育完整的叶绿体,在32°C下叶肉细胞数量及形态均正常。实时荧光定量PCR(qRT-PCR)分析表明,与野生型相比,tsa2突变体中部分光合色素代谢途径基因、叶绿体发育相关基因及光合作用相关基因的表达水平呈不同程度变化。遗传分析表明, tsa2突变表型受一对隐性核基因控制, TSA2被定位于第5染色体SSR标记S5-57和S5-119之间,物理距离为718 kb。本研究为水稻遗传改良及研究温度影响叶绿体发育机制奠定了基础。     

用于作物表型信息边缘计算采集的认知无线传感器网络分簇路由算法

随着无线终端数量的快速增长和多媒体图像等高带宽传输业务需求的增加，农业物联网相关领域可预见地会出现无线频谱资源紧缺问题。针对基于传统物联网的作物表型信息采集系统中存在由于节点密集部署导致数据传输过程容易出现频谱竞争、数据拥堵的现象以及固定电池的网络由于能耗不均衡引起监测周期缩减等诸多问题，本研究建立了一个认知无线传感器网络（CRSN）作物表型信息采集模型，并针对模型提出一种引入边缘计算机制的动态频谱和能耗均衡（DSEB）的事件驱动分簇路由算法。算法包括：（1）动态频谱感知分簇，采用层次聚类算法结合频谱感知获取的可用信道、节点间的距离、剩余能量和邻居节点度为相似度对被监控区域内的节点进行聚类分簇并选取簇头，构建分簇拓扑的过程对各分簇大小的均衡性引入奖励和惩罚因子，提升网络各分簇平均频谱利用率；（2）融入边缘计算的事件触发数据路由，根据构建的分簇拓扑结构，将待检测各区域变化异常表型信息触发事件以簇内汇聚和簇间中继交替迭代方式转发至汇聚节点，簇内汇聚包括直传和簇内中继，簇间中继包括主网关节点和次网关节点-主网关节点两种情况；（3）基于频谱变化和通信服务质量（QoS）的自适应重新分簇：基于主用户行为变化引起的可用信道改变，或分簇效果不佳对通信服务质量产生的干扰，触发CRSN进行自适应重新分簇。此外，本研究还提出了一种新的能耗均衡策略去能量消耗中心化（假设sink为中心），即在网关或簇头节点选取计算式中引入与节点到sink的距离成正比的权重系数。算法仿真结果表明，与采用K-medoid分簇和能量感知的事件驱动分簇(ERP)路由方案相比，在CRSN节点数为定值的前提下，基于DSEB的分簇路由算法在网络生存期与能效等方面均具有一定的改进；在主用户节点数为定值时，所提算法比其它两种算法具有更高频谱利用率。     

Salvianolate attenuates oxidative stress injury of human endothelial EA.hy926 cells induced by hydrogen peroxide

AIM: To investigate the effect of salvianolate on oxidative damage induced by hydrogen peroxide in human endothelial EA.hy926 cells.METHODS: EA.hy926 cells were cultured in vitro and divided into the following groups:control group, damage group, and anti-damage groups (salvianolate+damage groups). The cell viability was measured by CCK-8 assay. The migration ability of the EA.hy926 cells was detected by Transwell assay. The content of nitric oxide (NO) in the culture supernatant of the EA.hy926 cells was examined. The levels of vascular endothelial growth factor (VEGF) were detected by ELISA. The apoptosis,mitochondrial membrane potential and intracellular superoxide anion content of the EA.hy926 cells were analyzed by flow cytometry. The protein levels of caspase-3, cleaved caspase-3, Bcl-2, Bax, NF-κB and p53 were determined by Western blot. RESULTS: Compared with damage group, the viability of EA.hy926 cells pretreated with salvianolate at different concentrations was significantly increased (P<0.05). The apoptotic rate was significantly decreased (P<0.05). Savianolate enhanced the migration ability of the cells. The levels of VEGF, NO and mitochondrial transmembrane potential were increased (P<0.05), and the intracellular ROS level was significantly decreased (P<0.05). The protein levels of NF-κB, p53, Bax and cleaved caspase-3 were significantly decreased, and the protein level of Bcl-2 was markedly increased(P<0.05). CONCLUSION: Savianolate reduces the damage of EA.hy926 cells by hydrogen peroxide exposure, and its mechanism may be related to the blocking of NF-κB signaling pathway.     

樱桃番茄抗青枯病砧木新品种海茄砧1 号的选育

海茄砧1 号是以野生茄子自交系HZ09-5 为母本，以从越南引进的茄子品种自交系HZ10-2 为父本育成的高抗青枯 病樱桃番茄砧木品种。植株生长势较强，第1 雌花节位约为第7 节，花为紫色，果实卵圆形，青熟果淡绿紫色或淡绿色，果 萼绿色，果长7～9 cm，果宽4～6 cm，单果质量为50～60 g，种子千粒重为3.2 g 左右，种皮浅黄色，高抗青枯病。海茄砧 1 号与樱桃番茄的嫁接亲和性好，共生性强，嫁接苗成活率高。嫁接后的樱桃番茄果萼开展，果面有光泽，可明显改善果实 VC、可溶性固形物和可滴定酸含量等品质，提高产量。适宜华南地区樱桃番茄的嫁接栽培。     

A rapid,simple, and sensitive immunoagglutination assay with silica nanoparticles for serotype identification of Pseudomonas aeruginosa

An agglutination test based on colored silica nanoparticles (colored SiNps) was established to detect serotypes of Pseudomonas aeruginosa. Monodisperse colored SiNps were used as agglutination test carriers. The colored SiNps were prepared through reverse microemulsion with reactive dyes, sensitized with 11 kinds of mono-specific antibodies against P. aeruginosa, and denoted as IgG-colored SiNps. Eleven kinds of IgG-colored SiNps were individually mixed with P. aeruginosa on a glass slide. Different serotypes of P. aeruginosa could be identified by agglutination test with evident agglutination. The P. aeruginosa could be detected in a range from 3.6 × 10⁵ to 3.6 × 10¹² cfu mL^?1. This new agglutination test was confirmed to be a specific, sensitive, fast, easy-to-perform, and cost-efficient tool for the routine diagnosis of P. aeruginosa.     

Occurrence of prophage and historical perspectives associated with the dissemination of huanglongbing in mainland China

Huanglongbing (HLB), associated with a non-culturable bacterium ‘Candidatus Liberibacter asiaticus’ (CLas), is a highly destructive citrus disease with a long but poorly documented history in China. No effective treatment for HLB is available. The identification of new prophages in abundant CLas genomic sequence data provides new insights into both the diversity of CLas strains and HLB management. In this study, CLas populations from nine provinces were surveyed for the presence of prophage. Two major prophage typing groups (PTGs) were discovered to be associated with two different altitude regions: strains of CLas in PTG1 from high altitude regions (HAR) mainly contained prophage Type 1 only or Types 1 and 3, whereas strains of CLas in PTG2 from low altitude regions (LAR) mainly contained prophage Type 2. The discovery of these CLas population patterns provides evidence for independent origins of HLB in HAR and LAR. Guangdong province is the generally recognized domestic region of origin for HLB and is primarily responsible for the dissemination of HLB in LAR through transport of seedlings. Both Yunnan and Sichuan provinces are the probable regions of origin for HLB in HAR. PTG2 was further divided into two subgroups: PTG2-1, found in Guangdong, Fujian and Guangxi and PTG2-2, found in Jiangxi, Zhejiang and Hunan. These regions and prophage types are correlated with early and late introductions of HLB in LAR. These molecular analyses were supported by studying the history of the dissemination of HLB in historical documents.