利用CRISPR/Cas9系统检测果蝇细胞中组蛋白甲基化修饰对20E信号传导的调控

【目的】利用CRISPR/Cas9基因敲除系统在黑腹果蝇Drosophila melanogaster细胞中筛选并检测组蛋白甲基化修饰对蜕皮激素20 羟基蜕皮酮(20-hydroxyecdysone, 20E)信号传导的调控。【方法】通过Flybase网站分析并总结黑腹果蝇组蛋白甲基转移酶及其修饰位点;将5个组蛋白甲基转移酶基因［trr, Mes-4, ash1, Su(var)3-9和egg］的sgRNA插入到敲除载体pAc-sgRNA-Cas9骨架中并转染黑腹果蝇Kc细胞,利用TA克隆和测序鉴定突变位点。以Trr正调控20E初级应答基因Br-C的转录表达为阳性对照,利用qRT-PCR和Western blot检测该系统敲除靶基因的有效性;通过检测20E应答元件(20E response element, EcRE)双荧光素酶活性确定trr, Mes-4, ash1, Su(var)3-9和egg是否参与20E信号传导。【结果】果蝇组蛋白甲基化修饰主要发生在组蛋白H3的赖氨酸残基上,H3的精氨酸残基和组蛋白H4的甲基化修饰较少。trr敲除载体pAc-trr-sgRNA-Cas9转染Kc细胞后成功突变trr,降低H3K4三甲基化水平并阻断20E对其初级应答基因Br-C的转录诱导,证明该敲除系统的有效性。除trr之外,Mes-4和egg的敲除降低EcRE的双荧光素酶活性。【结论】插入靶标基因sgRNA序列的pAc-sgRNA-Cas9敲除载体在果蝇Kc细胞中可以有效快捷地突变靶基因。利用该敲除系统发现,除Trr之外,Mes-4和egg影响EcRE的活性而参与20E信号传导。本研究为昆虫细胞CRISPR/Cas9介导的基因敲除和组蛋白甲基化修饰调控20E信号传导的深入研究提供了理论依据与工作基础。     

柞蚕微粒子病潜在生物标志物的挖掘

【目的】挖掘柞蚕Antheraea pernyi微粒子病的潜在生物标志物,为开发该病害检测方法及研究柞蚕被微孢子虫Nosema pernyi侵染后体内代谢产物的差异及功能奠定基础。【方法】利用高效液相色谱和高分辨率质谱进行非靶向代谢组学分析,调查健康和患微粒子病柞蚕雌成虫血淋巴中代谢物差异。【结果】正离子模式下从健康和患微粒子病柞蚕雌成虫血淋巴中共获得8 870个代谢物,注释代谢物5 390个,筛选到差异表达代谢物472个(上调260个,下调212个),其中二级鉴定差异表达代谢物12个(上调8个,下调4个);负离子模式下获得6 716个代谢物,注释代谢物3 848个,筛选到差异表达代谢物301个(上调207个,下调94个),其中二级鉴定差异表达代谢物9个(上调8个,下调1个)。正离子模式下二级鉴定的差异表达代谢物包括缬氨酸(valine)、苯并噻唑(benzothiazole)、3-脱羟基肉碱(3-dehydroxycarnitine)、1 甲基鸟嘌呤(1-methylguanine)、2-乙氧基萘(2-ethoxynaphthalene)、N6-乙酰基-L-赖氨酸(N6-acetyl-L-lysine)、生物素(biotin)、桑色素(morin)、噻吗洛尔(timolol)、酰基肉碱15∶0(acylcarnitine 15∶0)、酰基肉碱18∶4(acylcarnitine 18∶4)和异槲皮苷(isoquercitrin);负离子模式下二级鉴定的差异表达代谢物包括二甲基丙二酸(dimethylmalonic acid)、戊二酸(glutaric acid)、2,5-二羟基苯甲酸(2,5-dihydroxybenzoic acid)、1,3-二乙酰基丙烷(1,3-diacetylpropane)、3-(4-羟基苯基)乳酸(DL-p-hydroxyphenyllactic acid)、泛酸(pantothenate)、荧光素(fluorescein)、飞燕草素-3-O-beta-吡喃葡萄糖苷(delphinidin-3-O-beta-glucopyranoside)和溶血磷酯酰肌醇16∶1 (lysoPI 16∶1)。【结论】健康与患柞蚕微粒子病的柞蚕雌成虫血淋巴内代谢物具有显著差异,通过代谢组学挖掘出21个二级鉴定的差异表达代谢物,这些代谢物可作为潜在生物标志物用于开发柞蚕微粒子病的检测方法。     

基于F3Net显著性目标检测的蝴蝶图像前背景自动分割

【目的】具有复杂背景的蝴蝶图像前背景分割难度大。本研究旨在探索基于深度学习显著性目标检测的蝴蝶图像自动分割方法。【方法】应用DUTS-TR数据集训练F³Net显著性目标检测算法构建前背景预测模型,然后将模型用于具有复杂背景的蝴蝶图像数据集实现蝴蝶前背景自动分割。在此基础上,采用迁移学习方法,保持ResNet骨架不变,利用蝴蝶图像及其前景蒙板数据,使用交叉特征模块、级联反馈解码器和像素感知损失方法重新训练优化模型参数,得到更优的自动分割模型。同时,将其他5种基于深度学习显著性检测算法也用于自动分割,并比较了这些算法和F³Net算法的性能。【结果】所有算法均获得了很好的蝴蝶图像前背景分割效果,其中,F³Net是更优的算法,其7个指标S测度、E测度、F测度、平均绝对误差(MAE)、精度、召回率和平均IoU值分别为0.940, 0.945, 0.938, 0.024, 0.929,0.978和0.909。迁移学习则进一步提升了F³Net的上述指标值,分别为0.961, 0.964, 0.963, 0.013, 0.965, 0.967和0.938。【结论】研究结果证明结合迁移学习的F³Net算法是其中最优的分割方法。本研究提出的方法可用于野外调查中拍摄的昆虫图像的自动分割,并拓展了显著性目标检测方法的应用范围。     

家蚕抗真菌因子BmSPI39对球孢白僵菌入侵的表达响应

【目的】制备家蚕Bombyx mori抗真菌因子BmSPI39的多克隆抗体,分析BmSPI39对球孢白僵菌Beauveria bassiana入侵的表达响应。【方法】利用原核表达和固定化镍离子亲和层析技术获得高纯度的BmSPI39重组蛋白,利用胶内活性染色检测重组蛋白BmSPI39对枯草杆菌Bacillus subtilis蛋白酶A的抑制活性;利用重组蛋白BmSPI39,通过免疫新西兰大白兔制备BmSPI39的多克隆抗体。基于家蚕开放性数据库SilkDB 3.0,分析BmSPI39在4龄第3天至化蛹后1 d家蚕免疫相关组织体壁、中肠和脂肪体中的时空表达特征。利用制备的BmSPI39抗体通过Western blot分析感染球孢白僵菌不同时间后家蚕幼虫和蛹体壁中BmSPI39应答球孢白僵菌入侵的表达响应。【结果】胶内活性染色结果显示,重组BmSPI39蛋白能够强烈抑制枯草杆菌蛋白酶A的活性。酶联免疫吸附结果显示,BmSPI39抗血清的抗体效价达1∶128 000。Western blot和胶内活性染色结果显示,纯化后的BmSPI39抗体能够有效结合不同多聚体化状态下的BmSPI39抗原蛋白。BmSPI39表达数据的热图分析显示,BmSPI39在游走期和预蛹期的家蚕体壁中有表达,在预蛹期的脂肪体中的表达量较高,但在各发育阶段的中肠中均不表达。Western blot分析结果表明,家蚕幼虫体壁中的BmSPI39的表达在感染球孢白僵菌后84 h上调表达,108和120 h下调表达。【结论】本研究成功制备了BmSPI39的多克隆抗体。BmSPI39蛋白的表达能够响应球孢白僵菌入侵,可能参与蛹期家蚕抵御真菌入侵的过程。     

西双版纳入侵长足捷蚁与土著黄猄蚁的种间竞争

【目的】入侵物种能够通过竞争影响本地物种的种群,从而影响入侵地的生物多样性。长足光捷蚁Anoplolepis gracilipes是全球最具破坏力的入侵蚂蚁之一。本研究旨在明确西双版纳地区入侵长足捷蚁与土著优势种蚂蚁黄猄蚁Oecophylla smaragdina之间的竞争关系。【方法】通过野外调查和室内控制试验相结合的方法,观察和对比分析长足捷蚁和黄猄蚁的体型大小,雾凉季和雨季的巢穴外觅食活动规律,觅食能力(搜寻食物的时间、在觅食时间内召集的最大工蚁数),打斗行为(不同打斗组合的攻击强度和死亡率)以及对饥渴的耐受性(无食物和水分供应时平均存活时间和存活率随时间的变化)。【结果】长足捷蚁工蚁体长(3.66±0.06 mm)显著小于黄猄蚁工蚁(8.27±0.16 mm)。在雾凉季时,长足捷蚁具有比黄猄蚁更长的觅食活动时间;而在雨季时,两种蚂蚁均在下午温度较高时段觅食活动的个体数量减少。苹果、蜂蜜和火腿肠3种食物作为诱饵时,长足捷蚁具有更快搜寻食物的能力,4~8 min便能找寻到食物,而黄猄蚁需要8~21 min才能找寻到食物,此外在寻找到食物后,长足捷蚁也有更快召集同伴的能力。在人工控制试验中,1头长足捷蚁和1头黄猄蚁同时存在时主要以不攻击和低强度攻击为主,而当两种蚂蚁中的任意其中一种的个体数量增加到5头时,攻击强度会显著增加,两种蚂蚁均存在种间协作行为。在饥渴状态下,两种蚂蚁工蚁的平均存活时间差异不显著,但长足捷蚁最长存活120 h,黄猄蚁最长存活96 h。【结论】在西双版纳地区,长足捷蚁相较于土著黄猄蚁具有更强的觅食的能力,雾凉季觅食活动时间更长,暗示长足捷蚁可能具有较强的温度适应能力。有必要加强对这一入侵蚂蚁的研究,并密切关注其种群在该地区的发展。     

家蚕5龄幼虫精巢和卵巢microRNA芯片及转录组比较分析

【目的】本研究旨在通过对家蚕Bombyx mori 5龄幼虫精巢和卵巢组织微小RNA (microRNA, miRNA)基因芯片及转录组进行分析,找到参与家蚕性腺发育相关的miRNA分子及可能的靶基因。【方法】采用新一代高通量测序平台对家蚕5龄幼虫精巢和卵巢(分别定义为Test和Control)进行miRNA基因芯片检测及转录组测序分析,根据P＜0.05且log₂(fold change, FC)≥2的标准,通过比较筛选出Test vs Control的差异表达miRNA;根据q≤0.05且|log₂(fold change)|≥1的标准,通过比较筛选出Test vs Control的差异表达基因 (differentially expressed genes, DEGs);随机选取8个上调和12个下调差异表达miRNA,对其表达及其预测的5个靶基因进行qRT-PCR验证;对DEGs以及差异表达miRNA的靶基因进行KEGG通路富集分析。【结果】从精巢和卵巢样本中(Test vs Control)分别鉴定出68个差异表达miRNA和3 991个DEGs,其中上调和下调miRNA分别为36和32个,上调和下调DEGs分别为2 033和1 958个。差异表达miRNA的qRT PCR验证结果均与芯片数据一致。KEGG通路富集分析结果显示DEGs在新陈代谢及核糖体的信号通路显著富集。对差异表达miRNA在DEGs中的可能靶基因进行预测,结果找到了4组表达趋势相反的miRNA与靶基因：分别是bmo-miR-2774a与LOC101745556;bmo-miR-92b与LOC101735954以及bmo-miR-3266与LOC733130和LOC778467;1组表达趋势一致的miRNA与靶基因：bmo-miR-3321与LOC101744895。5个靶基因的qRT-PCR验证结果与转录组测序结果一致。【结论】本研究获得了家蚕5龄幼虫精巢和卵巢转录组及miRNA芯片数据,筛选并验证了4组差异表达和1组一致表达miRNA及潜在靶基因,为探究家蚕精巢和卵巢发育差异奠定了基础。     

Effects of Exogenous Application of GA4+7 and NAA on Sugar Accumulation and Related Gene Expression in Peach Fruits During Developing and Ripening Stages

Sweetness is one of the key factors determining peach fruit quality. To better understand the molecular basis of gibberellic acid (GA) and 1-naphthaleneacetic acid (NAA) interference with sugar biosynthesis, a middle-late maturing commercial cultivar, ‘Jinxiu’ yellow peach fruit, was treated with three different concentrations of GA₄₊₇ and four of NAA. Fruit weight, firmness, total soluble solids, different sugar contents and the expression level of sugar-related genes were evaluated. The results showed that maximum increase in cv. ‘Jinxiu’ peach fruit size and sucrose content was with 1.25 mM GA₄₊₇, compared to control fruits and the other treatments during the ripening stages. The sucrose-phosphate synthase gene (PpSPS₂) which had a high level of expression and positive correlation with sucrose content was significantly regulated by 1.25 mM GA₄₊₇ in the final ripening stages. 0.5 mM NAA treatments significantly reduced the sucrose content and fruit size. Ninety percent of the fruits were deformed or dropped from the trees with treatments of 1 mM NAA and 2 mM NAA in the early development period. The crosstalk of different phytohormones and the related genes will be further investigated to get an insight into the inherent association between hormone control and sugar accumulation.

     

Effects of 5-HT7 receptors on circadian rhythm of mice anesthetized with isoflurane

ABSTRACT

The role of the serotonin 7 receptor (5-HT₇ receptor) subtype in a number of domains has been widely recognized, but its role in the regulation of changes of the circadian rhythm after anesthesia is still unclear. We used intraperitoneal injection of 5-HT₇ receptor agonist LP-211 or antagonist SB-269970 in mice to influence the level of 5-HT₇ receptor protein in the SCN and to observe the role of this receptor on circadian rhythm changes after isoflurane anesthesia. Our results show the appropriate dose of SB-269970 significantly alleviated the circadian rhythm disorder induced by isoflurane anesthesia, while LP-211 significantly aggravated it after anesthesia, which is different from the phase shift that can be caused by the administration of LP-211 before anesthesia. These findings may indicate the 5-HT₇ receptor plays a complex role in the regulation of circadian rhythm after anesthesia. Our findings may provide some positive significance for alleviating circadian rhythm disorder in patients after anesthesia and ultimately promoting rapid postoperative recovery.     

Inhibiting roles of FOXA2 in liver cancer cell migration and invasion by transcriptionally suppressing microRNA-103a-3p and activating the GREM2/LATS2/YAP axis

Cytotechnology - Forkhead box A2 (FOXA2) has emerged as a tumor inhibitor in several human malignancies. This work focused on the effect of FOXA2 on liver cancer (LC) cell invasion and migration...     

Offspring performance and female preference of Pagiophloeus tsushimanus (coleoptera: curculionidae) on three Lauraceae tree species: A potential risk of host shift caused by larval experience

The weevil Pagiophloeus tsushimanus Morimoto (Coleoptera: Curculionidae), native to Eastern Asia, is a wood-boring pest that causes severe damage to camphor trees (Cinnamomum sp.) in Shanghai, China. Other Lauraceae tree species that grew sympatrically with this pest in close proximity could face a potential threat. To assess the potential risks of host shift, we explored the phenotypic associations between preference and performance in P. tsushimanus reared on three Lauraceae tree species. In a no-choice experiment offering branches of each plant as diet material and oviposition sites, we found that individuals reared on Cinnamomum camphora (L.) Presl (Laurales: Lauraceae) exhibited the strongest performance with shorter development time, higher survival and growth rate in the immature stage, longer longevity and greater fecundity in adults. In contrast, those on novel Lauraceae tree species (Cinnamomum chekiangensis Nakai and Phoebe chekiangensis Shang) had difficulty completing their whole life cycle due to significantly lower survival and reproduction. In a multiple-choice experiment, C. camphora was established as the preferred host. However, we found that the larval experiences on the non-preferred host plants contributed to an increased preference for that plant species. These results indicated that both the preference-performance hypothesis and the Hopkins’ host selection principle are applicable in this weevil under experimental conditions. It is possible that although the weevil performed poorly on two novel Lauraceae tree species, under favourable conditions their surviving offspring could evolve into a new host-specific population. Consequently, this weevil pest needs to be monitored on these novel Lauraceae tree species.