保护地黄瓜新品种唐杂6 号的选育

唐杂6 号是以雌性系S16 为母本，以自交系S26 为父本配制的强雌型黄瓜一代杂种。生长势强，商品瓜短棒状， 瓜长12～14 cm，横径4.0～4.3 cm，非特异性环境下雌花率95% 以上，瓜皮嫩绿有光泽，白刺，刺瘤稀小，平均单瓜质量 131.8 g 左右，高抗霜霉病，抗细菌性角斑病，耐白粉病；春保护地栽培平均产量可达8 000 kg·（667 m²） ^-1，秋冬保护地栽 培产量可达6 500 kg·（667 m²） ^-1；适合河北、北京、天津及东北地区春、秋保护地种植。     

苦瓜新品种淮农青1号的选育

为了选育早熟、产量高、抗病性强、微苦的苦瓜新品种,以B19强雌系为母本,以B118苦瓜自交系为父本,进行杂交、分离后,经系统选育,培育出苦瓜新品种——淮农青1号。其早熟,果皮翠绿色,长纺锤形,口感脆嫩;前期平均667 m2产量1 126.2 kg,比对照增产25.5%,平均667 m~2总产量达2 740.8 kg,比对照增产26.3%;中抗白粉病,适合江苏省春季大棚栽培。     

京郊西兰花小菜蛾的田间防治药剂筛选与评价

为评价高效氯氰菊酯、溴氰虫酰胺、苏云金杆菌、甲氨基阿维菌素苯甲酸盐、乙基多杀菌素等5种杀虫剂对小菜蛾的田间药效,本文采用喷雾法进行了田间试验。结果表明,10%溴氰虫酰胺可分散油悬浮剂、6%乙基多杀菌素悬浮剂对小菜蛾在药后1~7 d的防效较好;32000 IU/mg苏云金杆菌可湿性粉剂、32000 IU/mg苏云金杆菌可湿性粉剂与10%溴氰虫酰胺可分散油悬浮剂分别按50%推荐用量组成的1∶1的混配剂,药后1 d的防效仅在60%左右,速效性较差,但是药后3~7 d的防效较好。其中,混配剂药后3 d的防效高达90.70%。5%甲氨基阿维菌素苯甲酸盐水分散粒剂和4.5%高效氯氰菊酯乳油在药后1~7 d的防效均较差。因此,在西兰花生产上可使用减量的溴氰虫酰胺与苏云金杆菌混配剂进行小菜蛾的防治,以达到农药减量增效防治小菜蛾的目的;在小菜蛾暴发时,可使用溴氰虫酰胺或乙基多杀菌素,以达到迅速防治的目的。     

白屈菜CmFAD2基因的克隆及植物转化载体构建

通过对白屈菜低温应答过程的转录组分析发现膜脂不饱和化相关基因的表达在一定过程中发生变化,脂肪酸去饱和酶基因FAD2在随温度的变化趋势为正"V"型,且表达量变化显著。利用NCBI等在线软件对序列进行相关生物学信息分析,并对白屈菜FAD家族成员FAD2基因的完整开放阅读框(ORF)进行克隆,并命名为CmFAD2。选用克隆载体pMD-19-T,转化大肠杆菌DH5α,测序验证序列正确性及完整性。将目的基因与植物表达载体pRI-201-AN连接构建重组DNA pRI-201-AN-Cm FAD2,电击法转化农杆菌LBA4404,利用菌液PCR法验证成功。该基因可作为药用植物抗寒品种创制的候选基因。     

马铃薯AP2/ERF转录因子的克隆及植物表达载体构建

AP2/ERF基因家族转录因子普遍存在于植物中,参与植物体内的各种生物学过程,包括植物的生长发育、生物和非生物胁迫响应等。前期转录组测序的结果发现马铃薯‘加湘1号’一个AP2/ERF家族基因(PGSC0003DMG400012154)在接种晚疫病菌(Phytophthora infestans)24 h后被显著激活。从接种P.infestans 24 h的‘加湘1号’的总RNA中通过RT-PCR获得了该基因CDS序列为885 bp,BLAST分析显示该基因编码一个295个氨基酸残基的蛋白,并且含有1个AP2/ERF结构域,是AP2/ERF转录因子家族中的ERF亚家族的一员。本研究将该基因与XcmⅠ酶切的表达载体pCXSN连接,转化大肠杆菌,通过测序挑选插入正确克隆酶切验证,并成功转化农杆菌。本研究结果为进一步研究该基因的功能提供了帮助。     

一个潜在催化莱鲍迪D苷合成的新型糖基转移酶

尿苷二磷酸糖基转移酶(uridine diphosphate glycosyltransferases,UGTs)催化糖基转移反应,与植物次生代谢密切相关。本研究根据甜叶菊(Stevia rebaudiana)转录组数据库,克隆到一个催化莱鲍迪D苷(rebaudioside D,RD)合成的新型糖基转移酶候选基因,对其开展生物信息学分析。结果表明,该基因开放阅读框长1380 bp,编码459个氨基酸,等电点(pI)预测为5.54,理论分子量约49.66 kD,系统发育分析表明该基因与向日葵中的UGT89A2同源,故将其命名为SrUGT89A2。构建pET28a-SrUGT89A2原核表达载体,并在大肠杆菌(BL21(DE3))中诱导表达得到重组蛋白,HPLC检测表明粗酶液能催化甜叶菊提取液形成一个新的色谱峰,该峰保留时间与莱鲍迪D苷一致。经进一步纯化UGT89A2蛋白,添加不同甜菊糖苷标准品为催化底物,但未鉴定出该蛋白催化的具体糖苷。该潜在催化甜菊糖RD苷合成的新型糖基转移酶基因SrUGT89A2的发现,为RD苷的生物合成和甜菊糖苷的生物途径研究提供新的理论依据。     

2018年中国部分地区猪瘟病毒2.1d亚型新流行株的基因组特征分析

为了解中国猪瘟病毒（classical swine fever virus，CSFV）的分子流行病学及遗传变异情况，本研究应用RT-PCR方法对2018年采集自河南、河北、山东、黑龙江和辽宁5个省份的350份疑似CSFV感染的病料进行E2和NS5B基因扩增，并对PCR产物进行测序和序列分析。结果显示，350份样品中21份为CSFV阳性，共获得14株CSFV的E2基因序列和7株CSFV的部分NS5B基因序列。E2全基因、NS5B部分基因序列分析表明，21份阳性样品均属于近年来在中国流行的CSFV 2.1d亚型，且新发现的2.1d亚型CSFV与中国较早2.1d亚型CSFV毒株间同源性差异不大，新发现的2.1d亚型CSFV分离株在E2基因的6个氨基酸（R³¹、S³⁴、W¹⁸²、K²⁰⁵、K³⁰³、A³³¹）上具有相同的分子特征，E2蛋白中15个位点上的半胱氨酸均未发生变异。韩国2.1d亚型CSFV在E2蛋白上具有3个独特的氨基酸（N⁹⁷、K¹⁵⁹、R²⁰⁵）特征，并且发现了韩国毒株YC11WB可能作为2.1b和2.1d亚型CSFV过渡毒株的证据，流行于中国和韩国的2.1d亚型CSFV可能分别来自于本国早期2.1b亚型CSFV的衍化。本研究证实，2018年中国及周边国家CSFV较为活跃，且流行毒株依然以2.1d亚型为主，为中国科学防控CSFV提供了依据。     

Dynamics of apoptosis-related gene expression during follicular development in yak

The potential reproduction power of domestic animals is limited by a complicated follicular atresia process. P53, caspase-9 (Casp9), Bax, Bcl-2 and Fas play a crucial role in the ovarian mitochondrion-dependent apoptosis and death receptor pathway. In accordance with this study, the expression levels of Casp9, Bax, Bcl-2 and Fas were analysed in ovaries and oviducts of yak by immunohistochemistry (IHC). P53 and the above in ovarian granulosa cells (GCs) from atretic (3–6 mm) to healthy follicles (6–8 mm) and in oviducts were examined from the luteal phase to the follicular phase during the oestrous circle by Western blot (WB) and real-time PCR (RT-PCR). Results demonstrated that typical classic apoptotic factors Casp9, Bax, Bcl-2 and Fas were expressed in the cytoplasm and zonal pellucida of oocytes, primordial follicles, primary follicles, ovarian surface epithelium, ovarian GCs, granular lutein cells, surface epithelia in oviduct uterotubal junction and oviduct ampulla during the luteal phase. RT-PCR and WB revealed that P53 and Fas significantly increased in GCs of atretic follicles. P53 and Casp9 increased in oviduct epithelium during the luteal phase, but Fas was unchanged. A contrary tendency was noted in Bcl-2 and Bax expression. Overall, P53 and Fas play an essential role in inducing GC apoptosis, and Bax, Bcl-2, Casp9 and P53 are involved in oviduct epithelial regeneration in yak.     

Knockdown of HMGA2 gene inhibits TGF-β1-induced human embryonic lung fibroblast growth and collagen synthesis

AIM: To investigate the effects of high mobility group A2(HMGA2) gene knockdown on the cell viability, apoptosis, collagen synthesis and oxidative stress of human embryonic lung fibroblast (HELF) induced by transforming growth factor-β1 (TGF-β1). METHODS: The HELF were divided into blank group, TGF-β1 group,negative control (NC) group and HMGA2 siRNA(si-HMGA2) group. The protein levels of HMGA2, AKT and p-AKT were determined by Western blot. The cell viability and apoptotic rate was analyzed by MTT assay and flow cytometry,respectively. The mRNA expression of collagen I (COL-Ⅰ) and COL-Ⅲ was detected by RT-qPCR. DCFH-DA was used to detect the content of reactive oxygen species (ROS). RESULTS: Compared with blank group, the protein levels of HMGA2 and p-AKT, the cell viability, the mRNA expression of COL-Ⅰ and COL-Ⅲ in TGF-β1 group were significantly increased, but the apoptotic rate and ROS level were significantly decreased (P<0.05). Compared with TGF-β1 group, the protein levels of HMGA2 and p-AKT, the cell viability, the mRNA expression of COL-Ⅰ and COL-Ⅲ in si-HMGA2 group were significantly decreased, but the apoptotic rate and ROS level were significantly increased (P<0.05). CONCLUSION: Knockdown of HMGA2 gene expression decreases the viability and collagen synthesis, and promotes apoptosis and ROS production of human embryonic lung fibroblasts induced by TGF-β1. The mechanism may be related to down-regulation of PI3K/AKT signaling pathway.