土霉素对柑橘黄龙病的防治效果及对柑橘产量和品质的影响

为有效防控柑橘黄龙病,于2017年在佛罗里达大学柑橘研究与教育中心的奥本代尔市柑橘试验场进行田间试验筛选黄龙病的防治药剂及其浓度,测定注射土霉素后叶片中柑橘黄龙病菌亚洲种Cadidatus Liberibacter asiaticus、土霉素、淀粉含量、柑橘产量、出汁率、可溶性固形物含量和酸度,显微镜下观察注射土霉素后淀粉粒的分布。结果表明,浓度为1.6g/株土霉素处理180 d后柑橘叶片中黄龙病菌亚洲种含量减少幅度最大,为91.78%;注射浓度为1.6g/株土霉素后7d,叶片中土霉素含量达142.2 μg/kg,注射后11 d叶片中土霉素含量达到最大,为239.8 μg/kg,注射后45 d叶片中土霉素含量低至99.6 μg/kg以下;注射后7~90d,叶片中黄龙病菌亚洲种含量呈波浪形变化,注射90 d后叶片中黄龙病菌亚洲种含量一直处于增长趋势,叶片中黄龙病菌亚洲种含量总体随着土霉素含量的升高而降低;注射浓度为1.6g/株土霉素后,叶片中淀粉含量大幅度下降,60d时达到最低值,为3.3 μg/mm²,90d时达到峰值,为14.5 μg/mm²;单株产量为16.7 kg,与注射浓度为0.8 g/株土霉素处理差异不显著,但均显著高于其它2个处理;柑橘出汁率、可溶性固形物和酸度均与清水对照差异不显著。表明土霉素可有效抑制黄龙病菌亚洲种,减少柑橘叶片内淀粉含量,增加柑橘产量,但对果实品质未产生显著影响。     

天维菌素酰化衍生物的合成及杀虫杀螨活性

以天维菌素B、天维菌素B单糖苷和天维菌素B苷元为原料,经选择性C-5羟基保护,在C-13、C-4′和C-4″位引入不同酰基基团,合成了3个系列共23个天维菌素B酰化衍生物,并通过1H NMR、13C NMR和高分辨质谱对所有目标化合物的结构进行了表征。生物活性测定结果表明,所有衍生物对小菜蛾Plutella xylostella、朱砂叶螨Tetranychus cinnabarinus以及松材线虫Bursaphelenchus xylophilus均表现出不同程度的毒杀活性,其中天维菌素B C-4″位衍生物的活性优于C-4′位衍生物及13位衍生物。化合物8e对小菜蛾和松材线虫的毒杀活性最优,LC50值分别为9.2 mg/L和0.42 mg/L,化合物8b对朱砂叶螨的毒性最高,LC50值为0.0019 mg/L,均优于对照药天维菌素B。     

呋喃磺草酮原药中主要杂质的结构鉴定及其合成

针对HPPD除草剂呋喃磺草酮原药生产中产生的3个质量分数均大于0.1%的主要杂质,通过高效液相色谱、核磁共振氢谱和高分辨质谱对3个杂质的结构进行了结构鉴定,发现其中2个为未见文献报道的化合物。结合生产工艺对杂质产生的路径进行了分析,并成功进行了合成。该研究对呋喃草酮原药质量控制和安全产生具有重要意义。     

水分和盐胁迫下小麦种子萌发相关性状的QTL定位

小麦萌发期对水分和盐胁迫敏感,对该时期水分和盐胁迫下种子萌发性状进行QTL定位具有重要的意义。本研究以小麦“泰农18×临麦6号” RIL群体为材料,以20%PEG-6000溶液和100 mmol·L^-1 NaCl溶液分别模拟水分和盐胁迫环境,对种子萌发期10个性状进行了QTL定位。结果表明,在正常、水分胁迫和盐胁迫3种不同处理下各性状变异较大。相关分析表明,抗旱和耐盐可能是两个独立遗传的性状,胚芽鞘长可以作为节水抗旱的鉴定指标。3种处理下共检测到10个萌发相关性状的103个QTL,其中,17个为相对高频QTL（RHF-QTL）,分布在7条染色体（1A、3A、3B、4B、7A、7B和7D）上,平均贡献率为7.55%~15.97%。这些RHF-QTL形成4个QTL簇（QTL cluster,QC）,分布在3A、7A和7D染色体上。其中,7A染色体上的QC2包括3个RHF-QTLs（ QSdw-7A.1、 QGf-7A.1和 QGi-7A.1）,均与小麦耐盐性相关;7D染色体上的QC3包括2个RHF-QTLs（ QGi-7D.1、 QGdrc-7D.1）,均与小麦节水抗旱性相关。这2个QCs增加效应均来自母本泰农18。本研究获得的RHF-QTLs和QCs,可为小麦萌发期节水抗旱和耐盐分子标记辅助选择提供理论和技术支持。     

Roles of protein phosphatase 4 in down-regulation of eNOS Ser633 phosphorylation induced by palmitic acid in human umbilical vein endotheli?al cells

AIMTo investigate the roles of protein phosphatase 4 (PP4) in down-regulation of endothelial nitric oxide synthase (eNOS) Ser633 phosphorylation induced by palmitic acid (PA). METHODSHuman umbilical vein endothelial cells (HUVECs) were treated with PA at 25 μmol/L, 50 μmol/L, 100 μmol/L and 200μmol/L for 36 h, or treated with PA at 100 μmol/L for 12 h, 24 h, 36 h and 48 h. Protein phosphatase 2A (PP2A) family inhibitor fostriecin (FST, 20 nmol/L) or okadaic acid (OA, 5 nmol/L) was selected to pretreat the HUVECs for 30 min. Protein phosphatase 4 catalytic subunit (PP4c) siRNA or protein phosphatase 2A catalytic subunit (PP2Ac) siRNA was transfected into the HUVECs. The protein expression levels of of eNOS, PP4c and PP2Ac, as well as the level of eNOS Ser633 phosphorylation, were detected by Western blot. The intracellular nitric oxide (NO) content was measured by DAF-FM DA. RESULTS(1) Compared with control group, the levels of eNOS Ser633 phosphorylation were decreased in PA groups in which the HUVECs were treated with 25 μmol/L, 50 μmol/L, 100 μmol/L and 200 μmol/L PA for 36 h (P<0.05) and 100 μmol/L PA for 24 h, 36 h and 48 h (P<0.05). No significant difference in the level of total eNOS protein expression among all the groups was observed. (2) Compared with control group, both FST and OA pretreatment reversed the reduction of eNOS Ser633 phosphorylation (P<0.05) and the decrease in intracellular NO content (P<0.05) induced by PA. No significant difference in the level of total eNOS protein expression among all the groups was observed. (3) Compared with si-Control group, the PP4c protein expression was significantly reduced (P<0.05), while the level of eNOS Ser633 phosphorylation was significantly increased in si-PP4c group (P<0.05). Although the levels of PP2Ac protein expression declined significantly (P<0.05), the level of eNOS Ser633 phosphorylation remained unchanged in si-PP2Ac group. No significant differencein the level of total eNOS protein expression among all the groups was found. CONCLUSION PA significantly reduces the level of eNOS Ser633 phosphorylation and the content of NO in the HUVECs, which may be due to PA inducing the activation of the PP2A family member PP4 rather than PP2A.     

Mechanism of elemene enhancing radiosensitivity of human glioma U251 cells

AIM To investigate the effect of elemene on the radiosensitivity of human glioma U251 cells and its mechanism. METHODS The U251 cells were used as a glioma model in vitro, and were exposed to different concentrations of elemene and different doses of radiation. The cell viability was measured by MTT assay, the apoptosis and cell cycle distribution were analyzed by flow cytometry, and the related protein levels were determined by Western blot. RESULTS Elemene inhibited the viability of U251 cells in vitro and enhanced the radiosensitivity of the cells. The cells in radiotherapy combined with elemene group had higher rates of early apoptosis, secondary necrosis and total cell death than those in radiation group. Elemene induced G₂/M phase arrest in the U251 cells. Elemene reduced the protein expression of cell division cycle protein 2 （Cdc2）, which resulted in the decrease in cyclin B1 expression induced by radiotherapy, thereby inhibiting the formation of cyclin B-Cdc2 complex. Elemene reduced Cdc2 activity by inhibiting the phosphorylation of Cdc2 protein at threonine 161, thereby inducing G₂/M phase arrest in the cells. It also mediated apoptosis by down-regulating survivin expression. CONCLUSION Elemene may increase the sensitivity of U251 cells to radiotherapy by down-regulating Cdc2 protein, decreasing cyclin B1 expression, inhibiting the formation of cylcin B-Cdc2 complex and down-regulating the expression of survivin.     

Effects of different active constituents of Gynostemma pentaphyllum on mitochondrial energy metabolism-related proteins in endothelial cells induced by ox-LDL

AIM To investigate the effects of different components of Gynostemma pentaphyllum ［gypenosides (Gps), gypenoside XLIX (GpXLIX) and ginsenoside Rb3 (GRb3)］ on mitochondrial energy metabolism-related proteins in endothelial cells induced by oxidized low-density lipoprotein (ox-LDL). METHODS EA.hy926 cells were divided into control group, model group, Gps group, GpXLIX group and GRb3 group. The cells in control group were cultured only in DMEM complete medium. The cells in model group were treated with 100 mg/L ox-LDL for 48 h. The cells in Gps group, GpXLIX group and GRb3 group were treated with 100 mg/L ox-LDL for 24 h, and then treated with Gps, GpXLIX and GRb3 at 100 mg/L for another 24 h, respectively. The ATP content in each group was detected by ELISA. The expression levels of mitochondrial energy metabolism-related proteins, cytochrome C oxidase subunit 5a （Cox5a）, NADH:ubiquinone oxidoreductase core subunit S1 （Ndufs1）, ATP synthase F1 subunit alpha (ATP5a) and cytochrome C (Cyt C）, were determined by Wes automatic Western blot quantitative analysis system and Western blot. RESULTS Compared with control group, the ATP content in model group was decreased (P<0.01). After drug intervention, the ATP content increased to different degrees in Gps group, GpXLIX group and GRb3 group (P<0.01). The results of Wes automatic Western blot quantitative analysis system were consistent with those of Western blot. These results showed that compared with control group, the protein expression of Cox5a, Ndufs1 and ATP5a in model group was decreased, and the protein expression of Cyt C was increased (P<0.01). After intervention, the protein expression of Cox5a, Ndufs1 and ATP5a was increased and the protein expression of Cyt C was decreased in Gps group, GpXLIX group and GRb3 group (P<0.05 or P<0.01). Among them, the effect of Gps on the protein expression of Cox5a, Ndufs1 and Cyt C was significantly stronger than those of the 2 monomer components, and the effect of GRb3 was found to be superior in the 2 monomer components. The effect of GpXLIX on ATP5a protein was superior to the other 2 components. CONCLUSION Gynostemma total saponins and related active ingredients protect ox-LDL-induced endothelial cells by affecting mitochondrial energy metabolism-related proteins, thereby preventing and treating atherosclerosis.     

虎雪兰玻璃化超低温法脱毒技术的研究

以兰属花卉虎雪兰组培原球茎为试材,采用玻璃化超低温法对兰花病毒脱除进行了研究,以期为虎雪兰玻璃化超低温法脱毒体系的建立提供参考依据。结果表明:在蔗糖浓度0.5 mol·L-1预培养4 d,然后在蔗糖0.6 mol·L-1加载液冰上处理50 min,之后转入PVS2溶液冰上玻璃化处理120 min,再液氮冷冻40 min,37℃水浴解冻3 min,最后卸载液(1/2MS+1.2 mol·L-1蔗糖)卸载20 min,待恢复培养后,原球茎成活率可达到65%以上,随机检测不同处理样品的脱毒率可达97%。     

3种引诱剂对松褐天牛成虫引诱效果比较

为了更好地对松褐天牛成虫进行监测和诱杀,在遂昌地区的马尾松林及贮木场内利用3种不同引诱剂对松褐天牛进行诱捕对比试验。结果表明,3种引诱剂对松褐天牛都有较好的引诱效果,但差异显著。其中,APF-Ⅰ型引诱剂的效果最好,F1型引诱剂次之,ST-2型最弱。试验期共诱捕到松褐天牛成虫4 979头,其中雌成虫4 134头,雄成虫845头,雌雄比为1∶0.204。所诱捕到的雌虫数量是雄虫的4.89倍,差异显著(P=0.045,t=-4.551)。引诱剂捕获松褐天牛的高峰期为6月中旬至8月中旬,6月至8月份降雨量及气温对松褐天牛成虫诱捕规律产生较大影响。本研究为遂昌地区松褐天牛成虫的防治提供了科学依据。     

风险感知、保险认知与养殖户肉鸡保险购买意愿 ——基于肉鸡主产区的实证分析

风险管理是现代农业经营中的重要问题,随着农业市场化程度的加深,肉鸡产业面临着多种风险来源的冲击。农业保险作为有效的现代风险管理工具,在保障产业可持续发展、减少农户家庭收入波动方面发挥了重要作用。基于行为金融理论,利用江苏、安徽、山东、河南和辽宁5个肉鸡主产区的调研数据,运用有序Logit模型,分析风险感知与保险认知对养殖户保险购买意愿的影响,探讨两者间的交互影响机制。结果表明,尽管66.43%的农户认为肉鸡养殖保险在风险管控中的必要性较强,但86.43%的农户对保险内容的了解程度不高,仅有20.71%的农户具有强烈的保险购买意愿。生产风险感知对养殖户的保险购买意愿有促进作用。保险认知中,农户对保险重要性认知程度对其保险购买意愿有促进作用;农户对保险内容的了解程度对其保险购买意愿具有显著的抑制作用,主要由于当前肉鸡保险产品设计不合理,保险内容与农户需求不匹配,保险理赔效果不佳,对保险内容了解程度越高反而会降低农户的购买意愿。风险感知和保险认知间存在交互影响,即风险感知对农户保险购买意愿的提高效果会随着对保险重要性认知程度的提高而增强,随着对保险内容了解程度的提高而减弱。因此,政府应加强农户的风险管理教育与培训,提高其风险管理意识,同时完善和优化当前肉鸡保险的内容,使之与农户需求相匹配,并通过更广泛的宣传来提高养殖户对于肉鸡保险的认知,从而增强农户对保险的购买意愿。