辣椒几丁质酶类基因家族的全基因组鉴定和表达特征分析

几丁质酶（chitinase, EC 3.2.1.14）是一种降解几丁质的糖苷酶,在植物应对非生物和生物胁迫中起重要作用。本研究对辣椒几丁质酶类（Capsicum annuum chitinase-like, CaCTL）基因家族成员进行了全基因组注释、进化分析和基因表达模式分析。从最新的辣椒基因组数据库中鉴定出31个CaCTL成员。根据系统发育进化树将这些成员分为GH18和GH19亚家族,并进一步分为5个亚类（Ⅰ~Ⅴ类）。保守基序分析结果表明,每个亚类中的成员存在功能相关性。对辣椒、矮牵牛以及番茄的CTL基因家族成员同源性分析表明,在矮牵牛和番茄中分别有7个和11个辣椒CaCTL的同源基因。通过qRT-PCR分析发现,在正常环境生长的辣椒植株中,64.2%的GH18亚家族的CaCTL成员表达水平很低,有64.7%的GH19亚家族成员在不同组织中存在差异表达。顺式作用元件分析表明,CaCTL成员启动子区域存在许多激素反应以及生物和非生物应激相关元件。当植物遭受不同的非生物胁迫时,qRT-PCR结果显示,多数CaCTL成员表达上调。当植物遭受高温干旱条件时,多个CaCTL成员的表达上调明显。上述结果丰富了CTL基因家族进化的研究,为探索CaCTL成员的功能提供了数据基础。     

生长素调控因子OsGRF4协同调控水稻粒形和稻瘟病抗性

【目的】水稻粒形为多基因控制的复杂数量性状,同时影响稻谷产量和稻米外观及碾磨品质,挖掘粒形相关基因并解析其遗传机制,对于水稻高产和优质品种选育具有重要意义。【方法】以前期利用大粒籼稻品种特大籼(TDX)为供体亲本、小粒粳稻品种日本晴(Nipponbare,NPB)为轮回亲本获得的一个大粒近等基因系,在水稻第2染色体上初定位粒形调控基因GS2.2(grain size 2.2)的基础上,对GS2.2基因进行了精细定位和候选功能基因的克隆鉴定。【结果】利用BC₄F₂群体中2887份极小粒单株及该群体中70份基因型杂合的大粒单株自交获得的BC₄F₃群体,将GS2.2基因精细定位在2M-7-1与2M-9之间的160.6 kb的区间内。该区间编码18个基因开放阅读框(ORF1-18)。测序发现ORF18基因在大粒近等基因系与小粒日本晴等位基因间存在5个SNP差异,ORF18编码生长素调控因子蛋白OsGRF4。采用CRISPR/Cas9基因编辑技术对大粒近等基因系中ORF18进行敲除,发现ORF18敲除株系粒长变短,证实ORF18是GS2.2的功能基因。进一步对ORF18大粒近等基因系和基因编辑敲除株系进行稻瘟菌室内离体和病圃接种鉴定,发现ORF18大粒近等基因系稻瘟病抗性增强,而基因编辑敲除株系稻瘟病抗性减弱,表明ORF18正调控水稻稻瘟病抗性。【结论】本研究发现的生长素调控因子OsGRF4协同调控水稻粒形和稻瘟病抗性,为协调水稻高产和抗性育种提供了重要的基因资源。     

Prevalence and antimicrobial resistance of Campylobacter from wild birds of prey in Spain

Wild birds have been identified as a relevant reservoir of Campylobacter spp., therefore, a potential source of infection in humans and domestic animals. The objective of this study was to determine the occurrence of Campylobacter spp. on birds of prey in Spain. In addition, antibiotic resistance profiles of the isolates were evaluated. A total of 689 specimens of 28 raptor species were analyzed, with a resulting individual prevalence of 7.5%. C. jejuni was the most frequently isolated species (88.5%), followed by C. coli and C. lari (3.8% each). The occurrence of Campylobacter was significantly higher (p < 0.05) in nocturnal birds of prey (15.3%), in spring season (12.2%) and in carnivorous species (9.4%). Isolates displayed a remarkable resistance to nalidixic acid (69.9%), ciprofloxacin (69.9%), and tetracycline (55.6%), and a low resistance to streptomycin (6.7%).Our findings highlight the importance of birds of prey as reservoirs of Campylobacter strains and their significant role as carriers of antimicrobial resistance.     

Transport of cadmium from soil to grain in cereal crops: A review

Due to rapid urbanization and industrialization, many soils for crop production are contaminated by cadmium(Cd), a heavy metal highly toxic to many organisms. Cereal crops such as rice, wheat, maize, and barley are the primary dietary source of Cd for humans, and reducing Cd transfer from soil to their grains is therefore an important issue for food safety. During the last decade, great progress has been made in elucidating the molecular mechanisms of Cd transport, particularly in rice. Inter-and intraspecific variations in Cd accumulation have been observed in cereal crops. Transporters for Cd have been identified in rice and other cereal crops using genotypic differences in Cd accumulation and mutant approaches. These transporters belong to different transporter families and are involved in the uptake, vacuolar sequestration, root-to-shoot translocation, and distribution of Cd. Attempts have been made to reduce Cd accumulation in grains by manipulating these transporters through overexpression or knockout of the transporter genes, as well as through marker-assisted selection breeding based on genotypic differences in Cd accumulation in the grains. In this review, we describe recent progress on molecular mechanisms of Cd accumulation in cereal crops and compare different molecular strategies for minimizing Cd accumulation in grains.     

牛星状病毒EvaGreen实时荧光定量PCR检测方法的建立及应用

牛星状病毒(BAstV)是我国新发的犊牛腹泻病原,本试验的目的是建立检测BAstV的Real-time PCR方法。根据BAstV流行株的ORF1a基因序列设计引物,通过优化反应条件和体系,成功建立基于EvaGreen检测BAstV的Real-time PCR方法。结果表明,该检测方法的Ct值与标准品模板在1.36×10¹~1.36×10⁸拷贝/μL线性关系良好,相关系数R²=0.999,扩增效率为93.79%;该方法可特异性检出BAstV,对犊牛腹泻其他相关病原呈阴性;最低检测下限为13.6拷贝/μL;批间和批内的变异系数均小于2%,重复性好。对2017年9月至2019年5月采自河南省的221份犊牛腹泻样本进行检测,BAstV的检出率为18.1%(40/221),采样场阳性率为100.0%(14/14)。本试验所建方法灵敏度高、特异性强、稳定性好,为BAstV的检测和流行病学调查提供了有力手段。     

生物多样性保护优先区生态网络构建与优化——以太行山片区为例

生物多样性保护优先区是重要物种的栖息地，是生物多样性保护工作的重点区域。基于生态学“源”“汇”理论，提取2000-2016年生态系统转移变化较小、生境质量较好的生态斑块和各类自然保护地作为生态源地，采用最小累积阻力模型构建研究区潜在生态廊道，并进行连通性评价，提出生态网络优化方案。结果表明，林地、灌丛是该区域物种迁移和扩散过程中起主导连接作用的景观类型，占生态廊道面积比例的63.9%，其次是草地，占生态廊道面积比例的13.87%；潜在生态网络结构连接度较高，但部分廊道结构较复杂，冗余性较高；通过重力模型优先选择相互作用力>5的生态廊道，并提取出32个生态断裂点和28个“暂栖息地”，最终提出保护生态源地、分级生态廊道、规划暂栖息地和修复生态断裂点等生态网络优化对策，研究结果可为太行山优先区-太行山片区生物多样性保护提供科学方法和建议。     

Bacteria and antibiotic resistance detection in fractures of wild birds from wildlife rehabilitation centres in Spain

Anatomic adaptations make birds more prone to open fractures with exposed bone parts losing vascularization. As a result of this exposure, fractures are colonized by different microorganisms, including different types of bacteria, both aerobic and anaerobic, causing osteomyelitis in many cases. For this reason, antibiotic treatment is common. However, carrying out antibiotic treatment without carrying out a previous antibiogram may contribute to increased resistance against antibiotics, especially in migratory wild birds. In this paper, bacterial counts regarding fracture type, bacterial identification and antibiotic resistance have been analysed in wild birds from wildlife rehabilitation centres in Spain. The results obtained showed that open fractures had higher bacterial counts (CFU/mL) than closed ones. Bacteria in family Enterobacteriaceae, identified were Escherichia spp., Enterobacter spp., Shigella spp., Hafnia alvei, Proteus mirabilis, Leclercia adecarboxylata and Pantoea agglomerans. Other bacteria present in wild birds’ fractures were Aeromonas spp., Enterococcus spp. Bacillus wiedmannii and Staphylococcus sciuri. All species found presented resistance to at least one of the antibiotics used. Wild birds can be implicated in the introduction, maintenance and global spreading of antibiotic resistant bacteria and represent an emerging public health concern. Results obtained in this paper support the idea that it is necessary to take this fact into account before antibiotic administration to wild animals, since it could increase the number of bacteria resistant to antibiotics.     

不同施氮水平对柳枝稷光合特性及抗旱性的影响

为了探究宁夏银北盐碱地区柳枝稷高产优质高效栽培过程中最佳的施氮量及其对柳枝稷叶片光合特性及抗旱性的影响,本研究采用大田试验,以Cave-in-Rock品种柳枝稷为供试材料,设无氮添加(0 kg·hm-2,N0)、施低氮(60 kg·hm-2,N60)、中氮(120 kg·hm-2,N120)和高氮(240 kg·hm-2,N240)共4个施氮水平,分析比较了各生育时期内柳枝稷叶片光合特性、渗透调节物质及抗氧化酶活性的变化,同时采用隶属函数法综合评价了盐碱地柳枝稷的抗旱性.结果表明,随着不同施氮水平的增加,柳枝稷各生育时期内叶片叶绿素相对含量(SPAD)、净光合速率(Pn)、气孔导度(Gs)和细胞间隙CO2浓度(Ci)整体呈现先升后降的趋势,均在施中氮(N120)处理下达到峰值.与无氮添加(N0)处理相比,施低氮(N60)、中氮(N120)和高氮(N240)处理下柳枝稷叶片的SPAD值平均增加了4.73％、18.71％和8.86％,净光合速率(Pn)平均提高了5.55％、17.02％和12.41％,气孔导度(Gs)平均升高了7.87％、56.18％和39.33％,细胞间隙CO2浓度(Ci)平均增加了7.86％、30.71％和13.81％.柳枝稷叶片蒸腾速率(Tr)在高氮(N240)处理下达到最大值,叶片水分利用效率(WUE)随着不同施氮水平的增加而逐渐下降.隶属函数分析结果表明,施中氮(N120)处理下柳枝稷各抗旱指标隶属函数值的均值最大.因此,本试验条件下有利于提高柳枝稷叶片光合能力和抗旱性的适宜施氮水平为120 kg·hm-2.     

绵羊心脏脂肪酸结合蛋白基因单核苷酸多态性分析

试验旨在探讨心脏脂肪酸结合蛋白（heart fatty acid-binding protein，H-FABP）基因在绵羊中的遗传多态性，并寻找可用于辅助选择的分子标记。本研究以滩羊（250只）及滩羊×湖羊杂交F1代（174只）为试验动物，利用SNaPshot分型技术对H-FABP基因（GenBank登录号：AY157617）的多态位点进行单核苷酸多态性（SNP）分析，统计基因频率和基因型频率，进行Hardy-Weinberg平衡性检测，计算期望杂合度（He）、多态信息含量（PIC）和有效等位基因数（Ne）等遗传多态指标，分析候选基因不同基因型与体重、体长、体高、胸围、胸深、胸宽和管围等生长性状的关联性。结果显示：①检测到9个多态位点：939[A/G]、980[G/A]、1018[T/C]、2878[C/T]、2956[C/T]、3017[G/A]、3341[G/C]、3394[T/A]、1056[-/G]，其中有6处转换、2处颠换、1处单碱基插入。②939[A/G]、980[G/A]、2956[C/T]、3341[G/C]、3394[T/A]和1018[T/C]的He为0.3200~0.4666，PIC为0.2688~0.3577；2878[C/T]、3017[G/A]位点的He为0.0283~0.1272，PIC为0.0279~0.1191，为低度多态；1056[-/G]位点的He在滩羊、滩羊×湖羊杂交F1代群体中分别为0.0120和0，PIC在滩羊、滩羊×湖羊杂交F1代群体中分别为0.0119和0；9个多态位点在滩羊、滩羊×湖羊杂交F1代群体中均符合Hardy-Weinberg平衡定律。③5个多态位点：939[A/G]、980[G/A]、2956[C/T]、3341[G/C]、3394[T/A]处于紧密连锁（D'>0.99），将H-FABP基因分为3个单倍型：AA、AB和BB。④在41只滩羊×湖羊杂交F1代羊中，BB单倍型在各生产性状上具有最大值，但各单倍型间差异不显著（P>0.05）。结果表明，绵羊H-FABP基因具有丰富的遗传多态性，939[A/G]、980[G/A]、2956[C/T]、3341[G/C]、3394[T/A]5个位点紧密连锁，BB单倍型可能是与绵羊生产性状相关的优势单倍型。     

水牛SND1基因克隆及生物信息学分析

试验旨在利用电子克隆法对水牛SND1（staphylococcal nuclease and tudor domain containing 1）基因进行克隆和序列分析，为探究该基因对水牛泌乳性能的作用机制奠定基础。以奶牛SND1基因（GenBank登录号：NM_205784.1）作为种子序列，利用Primer Premier 5.0设计3对引物，以水牛基因组DNA为模板，PCR扩增水牛SND1基因mRNA序列，扩增获得序列连接pMD18-T载体，通过测序拼接获得水牛SND1基因mRNA全序列，并对其进行生物信息学分析。结果显示，水牛SND1基因完整编码序列长为3 503 bp，包含长为2 733 bp CDS序列，编码910个氨基酸，蛋白分子式为C₄₅₂₃H₇₁₈₃N₁₂₈₁O₁₃₅₄S₂₆，分子质量为102.01 ku，理论等电点（pI）为6.74，不稳定系数为42.07，平均亲水性为-0.419，属可溶酸性蛋白。二级结构以α-螺旋和无规则卷曲为主，其中α-螺旋占37.80%，无规则卷曲占34.18%。结合Protfun 2.2在线软件对SND1的功能进行预测分析表明，该蛋白在嘌呤和嘧啶、中央中间代谢、能量代谢、氨基酸生物合成发挥功能的可能性分别为0.449、0.401、0.303和0.262。SND1基因编码区序列与黄牛、绵羊、山羊、猪、马、人的同源性分别为98.7%、97.8%、97.8%、93.8%、93.1%和91.7%，物种之间同源性较高，系统进化情况与其亲缘关系远近一致。利用SMART在线软件预测蛋白结构域，结果显示，水牛SND1蛋白包含有4个SN区域，说明SND1基因编码区在进化过程中较为保守。