水稻种子总RNA提取质量问题的探究

水稻种子总RNA提取在水稻分子遗传基础实验中起着非常重要的作用,然而,高质量水稻种子RNA的获取难度高,极大阻碍了cDNA文库构建、RNA-Seq和基因表达分析等相关研究工作的开展和深入。为了探讨水稻种子总RNA提取的相关影响因素,寻找合适的水稻种子总RNA提取方式,本研究通过比较Trizol法、GeneMark试剂盒法和艾德莱试剂盒法3种不同的提取方式、不同的耗材处理方法、研磨方式等不同因素改进水稻种子总RNA的提取效果。不同的检测结果显示,艾德莱多糖多酚提取试剂盒能够提取到28S、18S条带完整、降解少和纯度高的水稻种子总RNA;不同耗材处理方法中,蛋白酶K处理过的耗材提取的总RNA比另外两种方法处理过的耗材提取的总RNA降解更少,28S和18S条带更清晰和完整、总RNA质量最高、效果最好;而研磨方式上,液氮冷冻研磨法能够有效抑制RNA酶对RNA的降解。本研究对水稻种子RNA提取过程相关因素的分析和改进,为促进以水稻种子为研究对象的分子实验奠定了一定的技术基础。     

一株高病毒载量 PCV2 毒株的基因组特征及序列分析

【目的】了解广东省某猪群中猪圆环病毒 2 型（Porcine circovirus type 2,PCV2）流行毒株的遗传进化情况,丰富 PCV2 分子流行病学数据,为当地 PCV2 疫苗候选株的选用和研发提供参考。【方法】使用 qPCR 方法对疑似 PCV2 的样品进行检测,发现 1 株具有高病毒载量的 PCV2 毒株,命名为 GD222858。通过 PCR 方法进行全基因组分子克隆及遗传进化分析。使用 MegAlign 软件将该毒株 ORF1、ORF2 基因编码的氨基酸序列与 PCV2 同亚型参考毒株进行比对,分析氨基酸序列的相似性;采用 DNAStar 预测该毒株的 Cap 蛋白二级结构及 B 细胞表位,并与 4 株疫苗株 DBN-SX07-2（HM641752）、LG（HM038034）、SH（HM038027）、ZJ（AY686764）的 Cap 蛋白抗原指数进行比对分析。【结果】GD222858 毒株基因组长度为 1 767 bp。遗传进化分析表明该毒株属于 PCV2d 亚型。与国内外 82 株参考毒株的核苷酸相似性为 91.4%~99.6%,与越南毒株 Han8（GenBank 登录号：JQ181600）的亲缘关系最近。在 ORF1 编码的 Rep 蛋白处发现多个特异性突变位点 F70Y、F77L、W202R、N256S;ORF2 编码的Cap 蛋白相对保守。Protean 预测 Cap 蛋白的氨基酸第 5~18、24~25、39~41、48~49、57~65、99、101、112~114、139~140、145~150、162~165、175~181、188~189、205~211、227~232 位 置 处 均 可 能 存 在 潜 在 的 B 细 胞 表 位。GD222858 毒株的 Cap 蛋白抗原指数与 4 株疫苗株均有差异,在氨基酸 45~57、124~132、223~233 位置处抗原指数明显高于 4 株疫苗株,且与疫苗株 HM038034 差异最大。【结论】GD222858 毒株感染猪群的原因可能是 Rep 蛋白多个位点发生特异性突变及疫苗株选用不当所致。     

Uterine Expression of WNT7A and β-catenin After Induction of Oestrus in Sheep

WNT7A and β-catenin localisations and roles in regulating periimplantation ovine conceptus development under natural estrous conditions have been elaborated.However,their locations and expression patterns have not been reported under induction of oestrus.The localisation,expression and function of WNT7A and β-catenin in the uterine tissues of the early pregnant and non-pregnant sheep on days 10,12,14,16 and 18 following artificial induction of oestrus were investigated by means of in situ hybridisation,real-time RT-PCR,immuno-histochemistry and western blotting methods.WNT7A and β-catenin mRNA and protein were both restricted to the apical surfaces of the uterine luminal epithelium (LE) and glandular epithelium (GE).In pregnant sheep,protein localisation of WNT7A and β-catenin was observed both in the endometrial LE and GE.Their staining presented on day 10,increased between day 12 and day 16,and decreased on day 18.WNT7A and β-catenin mRNA and protein expression increased initially and then decreased from day 10 to day 18,peaking on day 16,and β-catenin reaching a peak on day 18 in the uterine tissues of pregnant sheep (p0.05).By contrast,no significant changes in WNT7A and β-catenin mRNA and protein expression levels were observed from day 10 to day 18 of the oestrus cycle in the uterine tissues of non-pregnant sheep (p0.05).Additionally,WNT7A and β-catenin mRNA and protein expression levels in the uterine tissues of the early pregnant sheep were significantly higher than those of non-pregnant sheep (p0.05).Treatment of endometrial epithelial cells with WNT7A increased the mRNA expressions of β-catenin,c-myc and Cyclin D1.These results provided an underlying mechanism of periimplantation ovine conceptus development under induction of oestrus.     

晚春造林技术研究

通过简单易行而有效的技术措施,成功试验且规模推广晚春造林技术,解决了当地春季火烧迹地更新造林季节脱节的矛盾。     

我国油菜品种改良现状及发展趋势

为了解我国油菜主导品种的品质发展现状和品种改良趋势,以“油菜品种改良”“油菜育种”“油菜产业发展”为关键词检索了PubMed、SpringerLink及中国知网等数据库,获得1987—2023年已发表的相关文献70篇,并结合农业农村部、国家统计局和中国种业大数据平台发布的油菜主导品种数据,综合分析我国油菜主导品种及产业现状、存在的风险与不足以及未来发展趋势。结果表明：1）我国油菜种植面积趋于稳定,油菜品种数量大幅增长,多样性更趋丰富;2）油菜主导品种含油率提升明显,且单产不断取得突破;3）当前我国油菜品种存在一些风险,如特专型品种含油率和产量较低、油菜品种同质化严重、抗病性不强、生育期短且抗逆性强的品种不足等。综上,我国油菜产业在品种改良和产业发展方面取得了显著进展,但仍需关注品种品质和抗病性等问题。未来可通过加强油菜种质资源收集与利用推进转基因生物育种的研发,推进油菜株型、抗性和光合效能的改造以实现产油率等一系列性状的再突破,满足多元化需求,探索密植增产技术,提升油菜机械化生产水平,推动我国油菜产业的可持续发展。     

Effect of Chitosan on Intestinal Bacteria of Allogynogenetic Crucian Carp,Carassius auratus gibelio,as Depicted by polymerase chain reaction‐denaturing Gradient Gel Electrophoresis

A 16S rDNA‐based polymerase chain reaction‐denaturing gradient gel electrophoresis (PCR‐DGGE) method was applied to detect intestinal bacterial communities of juvenile allogynogenetic crucian carp, Carassius auratus gibelio, fed with chitosan‐containing diet. This is the first time to use the molecular method to analyze the bacterial communities in the allogynogenetic crucian carp intestine. The DGGE profile with universal bacterial primers revealed simple communities in all treatment groups. Sequencing and phylogenetic analysis of excised DGGE bands showed that the dominant bacteria belonged to class γ‐Proteobacteria and Fusobacteria. The relative abundance and diversity of detected bacteria suggested that 0.5 and 0.75% of chitosan in diet were optimum for juvenile allogynogenetic crucian carp. As in these concentrations, some detected pathogen bacteria either disappeared or decreased. However, the DGGE profile with Aeromonas‐specific primers showed a similar composition among all treatment groups, which suggested that Aeromonas was one of relative stable bacteria components in the intestine of juvenile allogynogenetic crucian carp.     

关于公鱼属鱼类分类的讨论

本文回顾了公鱼属鱼类的分类历史,讨论了分类存在的问题,提出了赞同把该属分成形态特征和生态习性明显不同的两个种的意见:淡水产卵的定为池沼公鱼(H.olidus(Pallas),海水产卵的定为海公鱼(H.pretiosus(Girard)。     

江黄颡鱼人工繁育的初步研究

对江黄颡鱼人工繁殖和育苗进行了试验。以PG(鲤鱼脑垂体激素)、HCG(绒毛膜促性腺激素)等催产药物进行混合催产,水温24～26℃,效应时间为20～24h,产卵率为90%以上。采用等渗液稀释磨碎的精巢进行人工授精,用塑料网片着卵板粘卵,在孵化池内孵化,平均孵化率为87%。研究结果表明:江黄颡鱼在广西的适宜催产季节为4月中旬至6月底,工厂化育苗的饵料可用丰年虫和适口虾料来解决。     

鱼类特有的Ring型E3泛素连接酶MARCH5A基因在刺激隐核虫感染下的表达分析

为探究大黄鱼MARCH5A的免疫作用,实验采用反转录PCR确认了该基因的c DNA序列。该序列全长1045 bp,包含1个长度为867 bp的开放阅读框,编码288个氨基酸;序列分析显示该蛋白含1个RINGv和4个跨膜结构域。进化树分析表明大黄鱼有11个MARCH家族蛋白(与哺乳动物相同),但鱼类存在多个亚型,MARCH5A为鱼类特有蛋白,其蛋白理化性质和三维结构均与MARCH5B存在一定的差异。荧光定量PCR分析显示,MARCH5A在健康大黄鱼的多个组织中均有表达,在血液和心脏中表达量最高,其次为鳃和脑,而在肾脏和皮肤中表达量最少。刺激隐核虫感染大黄鱼后,MARCH5A在皮肤中早期表达量显著上调,第2天为对照组的9.65倍,后期下调。在鳃、脾脏和头肾中的前期表达量也有所增加,后期下降。结果表明大黄鱼MARCH5A在抗刺激隐核虫免疫应答过程中可能发挥重要作用。     

Molecular identification and genetic analysis for 24 turf-type Cynodon cultivars by Sequence-Related Amplified Polymorphism markers

Bermudagrass (Cynodon ssp.) germplasm is genetically diverse and widely distributed in the world. The study was conducted to identify and assess the molecular variation and relationship among 24 cultivars developed in China, Australia and the USA. Sequence-Related Amplified Polymorphism (SRAP) was applied to cultivars identification in this study for the first time. Thirty of the 90 SRAP primer combinations generated a total of 274 clearly bands encompassing 249 (91%) polymorphic. Each bermudagrass cultivar has its unique binary code and can be distinguished from the others. Three distinct clusters were obtained by unweighted pair-group method with arithmetic averages based on the polymorphic markers. Coefficients of genetic distance among the genotypes ranged from 0.57 to 0.97. The results demonstrated that SRAP marker is a stable molecular marker technique for the identification of bermudagrass cultivars and their genetic relationships.