Bamboo NiR gene is associated with regeneration capacity

It was reported that the activity of NiR (nitrite reductase) enzyme encoded by the NiR gene was correlated with the regeneration ability in rice. To testify the function of NiR gene in bamboo, seven bamboo species whose calli had different differentiation rate were chosen to analyse their NiR enzyme activity. The results showed that bamboo NiR enzymatic activity had a certain correlation with the regeneration capacity. A NiR gene named DhNiR from Dendrocalamus hamiltonii with high regeneration capacity was cloned. Sequence analysis revealed that the ORF of DhNiR was 1779bp encoding 592 amino acids. Overexpression of DhNiR in rice reduced the time of shoot differentiation and increased the transformation rate, suggesting that DhNiR might play an important role in the regeneration ability of bamboo, and can be applied in regeneration and gene transformation of bamboo and other plant species.     

Immunostimulatory effects of dietary poly‐β‐hydroxybutyrate in European sea bass postlarvae

The stable production of high‐quality fry in marine aquaculture is still hampered by unpredictable mortality caused by infectious diseases during larval rearing. Consequently, the development of new biocontrol agents is crucial for a viable aquaculture industry. The bacterial energy storage compound poly‐β‐hydroxybutyrate (PHB) has been shown to exhibit beneficial properties on aquatic organisms such as enhanced survival, growth, disease resistance and a controlling effect on the gastrointestinal microbiota. However, the effect of PHB on the developing immune system of fish larvae has so far not been investigated. In this study, the effect of feeding PHB‐enriched Artemia nauplii on survival, growth and immune response in European sea bass (Dicentrarchus labrax) postlarvae was examined. Amorphous PHB was administered to 28‐day‐old sea bass postlarvae over a period of 10 days. The survival and growth performance were monitored, and the expression of 29 genes involved in immunity, growth, metabolism and stress‐response was measured. While the expression of the insulin‐like growth factor 1 (igf1), an indicator of relative growth, was upregulated in response to feeding PHB, the larval survival and growth performance remained unaffected. After 10 days of PHB treatment, the expression of the antimicrobial peptides dicentracin (dic) and hepcidin (hep) as well as mhc class IIa and mhc class IIb was elevated in the PHB fed postlarvae. This indicates that PHB is capable of stimulating the immune system of fish early life stages, which may be the cause of the increased resistance to diseases and robustness observed in previous studies.     

Molecular cloning and functional characterization of the fatty acid delta 6 desaturase (FAD6) gene in the sea cucumber Apostichopus japonicus

The sea cucumber (Apostichopus japonicus), an important echinodermata, had high value in nutrition and medicine for its rich collagen, sulphated polysaccharide, glycosides and polyunsaturated fatty acids (PUFA). The cDNA of the fatty acid desaturase gene in A. japonicus (AJFAD6) was cloned and was found to encode a desaturase with delta 6 FAD activity. Sequence analysis indicated that AJFAD6 included an open reading frame of 1392 bp, encoding 463 amino acids. AJFAD6 has all the conserved motifs found in other members of the FAD6 family, including an N‐terminal cytochrome b5 domain and three histidine‐rich regions. qRT‐PCR showed that AJFAD6 was expressed in all tissues tested during juvenile development and was mainly expressed in the respiratory tree at 150 days after adherence (150 days) and in the intestine at 100 days. Furthermore, AJFAD6 mRNA was also detected in the analysed adult tissues, with higher expression in the intestine and testis. Functional characterization of AJFAD6 in a recombinant yeast, Pichia pastoris, showed that AJFAD6 could catalyse exogenous linoleic acid (LA) and α‐linolenic acid (ALA) to produce γ‐linoleic acid (GLA) and stearidonic acid (STA), respectively, at conversion rates of 11.1% for LA to GLA and 3.4% for ALA to STA. Our results suggested that the biosynthetic pathway of PUFA existed in the sea cucumber, but endogenous production of eicosapentaenoic acid, arachidonic acid and docosahexaenoic acid from either LA or ALA precursor appeared to be limited.     

茶树牻牛儿基牻牛儿基焦磷酸合成酶基因CsGGDPS的克隆及表达分析

以铁观音芽叶为材料,验证从茶树转录组数据库中筛选到的1条牻牛儿基牻牛儿基焦磷酸合成酶(GGDPS)的编码全长序列c DNA。该c DNA全长1 661 bp,含有1个1 137 bp完整的开放阅读框,命名为Cs GGDPS。该基因编码378个氨基酸,氨基酸序列具有类异戊二烯合成酶家族的5个保守域和2个特征功能域;序列分析显示,该c DNA与其他植物GGDPS高度保守,与三七(Panax notoginseng)的亲缘关系最近。Cs GGDPS属于不稳定、亲水蛋白,可能定位到叶绿体中,不存在跨膜结构,无信号肽,发生磷酸化的位点可能有20个;二级结构主要由α-螺旋构成,三级结构与拟南芥GGPPS11匹配度最高。实时荧光定量PCR结果表明,在茶树发育过程和不同叶位Cs GGDPS的表达量随芽叶成熟度的增加呈上升趋势,随着做青过程的进行,Cs GGDPS的表达量逐渐升高;Cs GGDPS在父本黄旦、母本铁观音和子一代金观音中均有表达,但表达量存在差异。     

三种因素对海水生物流化床启动期间营养盐去除及amoA基因表达的影响

在实验室规模下,以旋转式生物流化床(CB-FSB)为研究对象,研究了初始总氨氮(TAN)、水温及滤料膨胀率3种条件下,海水生物流化床生物过滤功能启动期间TAN和亚硝酸盐氮(NO-2-N)去除及amoA基因数量的变化。结果显示:生物流化床生物过滤功能启动所需时间随着水温的升高而缩短,在水温为15℃、20℃和25℃时,启动所需时间分别为27 d、25 d和23 d;初始TAN质量浓度的升高也会缩短生物流化床生物过滤功能启动所需要的时间,在初始TAN质量浓度为1 mg/L、2 mg/L、4 mg/L时,启动所需时间分别为24 d、22 d和21 d;在膨胀率为100%和150%时,启动所需时间无明显差别,分别为21 d和20 d,明显好于膨胀率为50%时启动所需时间27 d;amoA基因的数量变化与TAN去除率的变化有一定的相关性,并随着初始TAN浓度的升高而增多,在4 mg/L时数量最多,达到2.76×10~7copies/g。     

大豆Abhydrolase_3基因家族进化分析

异黄酮是大豆的重要次生代谢物,参与植物与微生物互作。2-羟基异黄酮脱水酶(hydroxyisoflavanone dehydratase,HID)催化2-羟基异黄酮形成稳定的异黄酮。HID属于Abhydrolase_3基因家族,该基因家族具有多种功能,但该基因家族在大豆中的进化模式尚待研究。为了研究Abhydrolase_3基因家族在大豆中的进化模式,本文在大豆基因组中鉴定了62个Abhydrolase_3基因,串联和片段复制是该基因家族主要扩增方式。根据系统进化关系,将大豆Abhydrolase_3基因家族划分为8个亚家族,其中HID所在的亚家族I基因数量最多,并发生多次基因扩增事件。对大豆Abhydrolase_3基因家族结构分析表明,不同亚家族具有不同的基序。多态性分析表明,亚家族Ⅰ、Ⅲ和Ⅴ具有较高的核苷酸差异,并受到放松的自然选择。基因表达分析表明,除了亚家族II和IV外,其它亚家族的基因在大豆不同组织中有较高表达;亚家族Ⅰ、Ⅲ、Ⅳ、Ⅴ和Ⅵ基因受病原菌诱导表达。结果说明HID所在的亚家族I存在基因扩增和功能分化,与病原菌互作相关的基因具有较高的遗传多样性并受病原菌诱导表达。     

大豆PAL2-3基因的克隆及转化研究

大豆异黄酮是苯丙氨酸代谢途径中合成的一类次级代谢产物,在苯丙氨酸代谢途径中,苯丙氨酸解氨酶(PAL)是关键酶和限速酶。本课题组前期研究发现PAL基因的相对表达量与大豆异黄酮含量具有明显的协同增减趋势,并且在PAL基因家族成员时空表达模式分析中发现,PAL2-3(XM_003542493)是PAL基因家族中相对表达量较高的主要表达成员之一。本试验首先通过克隆大豆中PAL2-3基因;然后构建pCAMBIA3301-GmPAL2-3植物过表达载体,将构建好的pCAMBIA3301-GmPAL2-3表达载体重组质粒转化到根癌农杆菌EHA105中;采用农杆菌介导的大豆子叶节转化体系获得转化植株,并对T1代转化植株进行PPT检测,外源标记基因Bar检测以及荧光定量PCR检测,对转基因阳性植株进行大豆籽粒异黄酮含量的测定。结果表明T_1代转基因植株中PAL2-3基因的表达量是对照的5.11~11.24倍,总异黄酮含量最高的(2 587.63μg·g~(-1))是对照(1 616.90μg·g~(-1))的1.6倍。因此在大豆中过量表达PAL2-3基因可以提高大豆籽粒中异黄酮含量。     

Seedling and adult plant resistance to leaf rust in 46 Chinese bread wheat landraces and 39 wheat lines with known Lr genes

Wheat leaf rust,caused by Puccinia triticina(Pt),is an important foliar disease that has an important influence on wheat yield.The most economic,safe and effective way to control the disease is growing resistant cultivars.In the present study,a total of 46 wheat landraces and 34 wheat lines with known Lr(leaf rust resistance)genes were inoculated with 16Pt pathotypes for postulating seedling resistance gene(s)in the greenhouse.These cultivars and five wheat differential lines with adult plant resistance(APR)genes(Lr12,Lr22b,Lr34,Lr35 and Lr37)were also evaluated for identification of slow rusting resistance in the field trials in Baoding,Hebei Province of China in the 2014–2015 and 2015–2016 cropping seasons.Furthermore,10 functional molecular markers closely linked to 10 known Lr genes were used to detect all the wheat genotypes.Results showed that most of the landraces were susceptible to most of the Pt pathotypes at seedling stage.Nonetheless,Lr1 was detected only in Hongtangliangmai.The field experimental test of the two environments showed that 38 landraces showed slow rusting resistance.Seven cultivars possessed Lr34 but none of the landraces contained Lr37 and Lr46.Lr genes namely,Lr9,Lr19,Lr24,Lr28,Lr29,Lr47,Lr51 and Lr53 were effective at the whole plant stage.Lr18,Lr36 and Lr45 had lost resistance to part of pathotypes at the seedling stage but showed high resistance at the adult plant stage.Lr34 as a slowing rusting gene showed good resistance in the field.Four race-specific APR genes Lr12,Lr13,Lr35 and Lr37 conferred good resistance in the field experiments.Seven race-specific genes,Lr2b,Lr2c,Lr11,Lr16,Lr26,Lr33 and LrB had lost resistance.The 38 landraces showed slow rusting resistance to wheat leaf rust can be used as resistance resources for wheat resistance breeding in China.     

桃蚜电压门控钠离子通道基因cDNA克隆及其生物信息学分析

克隆获得桃蚜电压门控钠离子通道基因cDNA序列，明确钠离子通道的典型特征，为研究桃蚜抗性分子机理奠定基础。采用实验技术主要有RT-PCR和PCR，克隆桃蚜钠离子通道基因cDNA序列，利用相关软件对其序列进行生物信息学分析。克隆得到两段cDNA序列MpNa_v-1（NCBI登录号：MN124170）和MpNa_v-2（NCBI登录号：MN176136）。MpNa_v-1长度为2945 bp，包括2877 bp的完整开放阅读框，共编码958个氨基酸；MpNa_v-2长度为3546 bp，包括3486 bp的完整开放阅读框，共编码1161个氨基酸。MpNa_v-1和MpNa_v-2共同组成桃蚜的钠离子通道α亚基，MpNa_v-1包含同源结构域Ⅰ和同源结构域Ⅱ，MpNa_v-2包含同源结构域Ⅲ和同源结构域Ⅳ。同源比对发现，桃蚜与豌豆蚜和高粱蚜钠离子通道基因相似度分别高达97.67%和97.65%，所克隆序列包含昆虫钠离子通道α亚基典型特征，具有MFM模块，并含有蚜虫类钠通道特有模块DENS。成功地克隆桃蚜钠离子通道基因，为阐明其对拟除虫菊酯类药剂产生靶标抗性的分子机制奠定基础。     

茶足柄瘤蚜茧蜂脂代谢相关的滞育关联基因差异表达分析

本文对茶足柄瘤蚜茧蜂滞育组与正常发育组进行转录组测序，筛选差异表达基因，根据功能注释发现这些滞育关联基因主要与碳水化合物代谢、脂质代谢以及信号转导等途径相关。借助KEGG数据库，共筛选出滞育期间401个与脂代谢相关的差异基因，在滞育期间呈现不同程度的上调表达，涉及了脂肪酸生物合成、甘油脂代谢、类固醇生物合成等代谢途径，除与脂质合成相关的脂肪酸合成酶、超长链脂肪酸延伸酶基因上调表达外，与脂质分解相关的酶，如酯酶同样上调表达，可能与提高茶足柄瘤蚜茧蜂免疫力有关；与激素合成相关基因的上调表达，可能抑制茶足柄瘤蚜茧蜂卵巢发育。