新生隐球菌RBP1基因克隆与功能分析

新生隐球菌是自然界广泛存在的具荚膜的酵母型病原真菌,能侵染人类中枢神经系统引起真菌性脑膜炎,每年导致全球大约18万人死亡。本研究在前期隐球菌交配表达谱的基础上,选择一上调表达的RNA结合蛋白基因（CNAG_04772）,进行克隆和功能分析。结果表明该基因全长2 247bp,cDNA全长1 518bp,编码505个氨基酸组成的蛋白,含有2个RNA识别基序RRM1和RRM2,命名为RBP1。基因表达模式分析表明RBP1在隐球菌酵母细胞、担子以及担孢子阶段都有表达,交配菌丝阶段不表达;亚细胞定位分析表明Rbp1蛋白定位于隐球菌的细胞核和细胞质中。与野生型菌株H99相比,敲除突变体菌株能够交配并产生双核菌丝,但丧失产生担孢子的能力,而互补菌株与野生型菌株H99间无显著差异。致病力测定结果显示,敲除突变体菌株致病性显著降低。     

模拟氮沉降和干旱对准噶尔盆地两种一年生荒漠植物生长和光合生理的影响

氮素和水分是荒漠生态系统的两个主要限制因子, 研究两者对荒漠植物的效应有助于深入了解荒漠生态系统对全球变化的响应。该文选择准噶尔盆地荒漠地区两种常见的一年生植物涩荠(Malcolmia africana)和钩刺雾冰藜(Bassia hyssopifolia), 设置0、0.18和0.72 g N·m ^-2·week ^-13个施氮浓度和湿润与干旱两个土壤水分处理, 研究模拟氮沉降增加和干旱对其生长和光合生理的影响。结果表明: (1)两种植物的根长、根重、叶片数、叶面积、总生物量和冠根比均随着施氮浓度的增加而增加, 干旱能够抑制氮对植物生长的促进作用, 但是, 氮的增加同时也能部分缓解干旱对植物生长的影响。与钩刺雾冰藜相比, 涩荠的根长、生物量和冠根比更易受氮增加和干旱的影响。(2)两种植物的最大净光合速率、叶绿素含量、可溶性蛋白含量随着氮浓度增加而增加, 但涩荠和钩刺雾冰藜对氮增加和干旱的生理响应也有所不同, 涩荠的响应更加敏感。两种植物对氮沉降和干旱胁迫响应的差异可能是其生活型等生物学特性差异所引起。通过对两种一年生植物的生长和光合生理分析表明, 在古尔班通古特沙漠, 春季丰富的降水和氮素增加将有利于涩荠和钩刺雾冰藜的生长和生产力的增加, 相对地下生长, 地上部分增加更显著。当干旱季节来临时, 氮的增加又能够在一定程度上降低干旱对这两种植物的负效应, 说明其对干旱具有一定的生态补偿作用。     

一种经microRNA敲低PD-1的新型慢病毒载体在CAR-T细胞中的应用

本研究将microRNA插入EF1α启动子的内含子中,构建携带沉默PD-1基因的miRNA的新型慢病毒载体,并将其应用于CAR-T细胞。通过流式细胞术检测慢病毒载体转导效率和PD-1沉默效率;Westernblotting检测PD-1蛋白表达差异;荧光定量PCR检测microRNA相对表达情况;荧光素酶生物发光法和流式细胞术检测CAR-T细胞的能力。结果显示与U6转录microRNA的载体相比较,将microRNA插入到EF1-α内含子中的病毒载体转导效率更显著,对PD-1的敲低效率均达90%以上,且Westernblotting结果验证了PD-1的敲低效果。另外通过荧光定量PCR,可显示出转导该新型慢病毒载体的Jurkat细胞内microRNA的相对表达量。荧光素酶生物发光法证实了CAR-T细胞针对靶细胞的特异杀伤性,流式细胞术结果表明沉默PD-1的CAR-T细胞相较于正常CAR-T细胞显示出更强的特异性杀伤能力。本研究成功构建了经microRNA敲低PD-1的新型慢病毒载体并验证了其转导效率的优越性,以及基于此载体表达的microRNA可高效地沉默PD-1;且应用此载体的CAR-T细胞能发挥更强的杀伤活性,从而为后续该CAR-T细胞治疗表达PD-L1的肿瘤奠定基础。     

停乳链球菌isp基因的克隆与原核表达

根据GenBank报道的停乳链球菌(Streptococcus dysgalactiae)isp基因(GenBank:CP002215.1)序列设计引物,PCR扩增得到isp基因。片段大小为1 500 bp,与从GenBank下载的序列进行同源性比对结果为98.57%。将isp基因克隆于表达载体pET-25b,成功构建了重组质粒pET-25b-isp,将重组质粒分别转化BL21(DE3),将BL21(pET-25b-isp)阳性重组菌株经IPTG诱导后,SDS-PAGE结果显示均有蛋白表达,大小分别为53 ku与目的蛋白大小相符;Western blot检测显示,表达的蛋白为目的蛋白。对成功构建的菌株BL21(pET-25b-isp)表达条件经优化后,在温度37℃,诱导时间12 h,IPTG浓度为1 mmol/L时,蛋白有较高的表达量。     

中华倒刺鲃幼鱼饲料蛋白质需求量的研究

以白鱼粉为蛋白源,设计了6个不同蛋白质含量(20.49%、26.48%、34.20%、41.02%、49.94%和55.86%,分别表示为D1、D2、D3、D4、D5和D6)的等能饲料,采用室内循环水养殖系统,在水温为(27.5±0.5)℃的条件下对中华倒刺鲃幼鱼进行10周的养殖实验,探讨中华倒刺鲃幼鱼对饲料蛋白质的需求量。每个处理设4个重复,每个重复12尾鱼。结果显示：干物质摄食率(FRdm)随饲料蛋白质含量升高呈先降低然后稳定的趋势;蛋白质摄食率(FRp)与饲料蛋白质含量呈正相关关系(r=0.982,p<0.01)。干物质表观消化率随饲料蛋白质含量增加而降低,蛋白质消化率在各组间无显著差异。随饲料蛋白质含量由D1逐渐增加至D4,体重特定生长率(SGRw)、能量特定生长率(SGRe)和饲料效率(FE)均显著增高(p<0.05),而D4、D5和D6组间无显著差异,其中D4组的三个指标值均最高,分别为(0.97±0.04)%/d、(0.87±0.04)%/d、(68.96±3.00)%。蛋白质效率(PER)、蛋白质累积率(PPV)和能量累积率(EPV)在各饲料组间均存在显著差异。以SGRw、SGRe和FE为指标,采用折线模型分析表明,中华倒刺鲃幼鱼的最适饲料蛋白质含量为39.6%－42.2%。     

序列特异的三锌指多肽的构建及其在大肠杆菌中的表达

在获得单一锌指突变体的基础上,以小鼠转录因子Zif268的三锌指DNA结合区为模板,利用重叠(Over-lap)PCR技术,获得了关键氨基酸位点同时突变的三锌指突变体ZF123、2ZF123。ZF123、2ZF123分别克隆进pUC-18质粒,序列测定正确后,以pGEX-2T为表达质粒,在大肠杆菌JM109中实现了功能性的表达。经SDS-PAGE分析,表达出了分子量34.0kD的融合蛋白,扫描分析其含量在20%左右。菌体经超声波破碎后,对可溶性融合蛋白进行了纯化得到了游离的目的蛋白,为进一步的DNA结合特性分析、杂交转录因子的构建等奠定了基础。     

木聚糖酶与XIP型木聚糖酶抑制蛋白相互作用分子机制的研究进展

Xylanase inhibitor protein (XIP)型木聚糖酶抑制蛋白对大部分GH10、GH11家族的真菌木聚糖酶具有抑制作用,但是却不能抑制细菌来源和植物自身所产生的木聚糖酶。XIP型木聚糖酶抑制蛋白对木聚糖酶的抑制作用主要是通过模拟底物接触酶的活性位点,迅速阻塞底物进入活性位点区域的通道。然而,在对XIP型木聚糖酶抑制蛋白具有抗性的GH10和GH11木聚糖酶晶体结构中,连接二级结构的Loop构象严重阻碍了XIP型木聚糖酶抑制蛋白的抑制功能。与对XIP型木聚糖酶抑制蛋白敏感的木聚糖酶相比,氨基酸残基的插入突变导致抗性木聚糖酶的Loop具有明显的凸出构象;而在GH11家族抗性木聚糖酶中,"拇指"结构中部分氨基酸的替换致使XIP型木聚糖酶抑制蛋白与"拇指"结构无法形成稳固的氢键和疏水建,从而削弱XIP的抑制作用。     

Leek Yellow Stripe Virus Can Adjust for Host Adaptation by Trimming the N-Terminal Domain to Allow the P1 Protein to Function as an RNA Silencing Suppressor

In Japan, the P1 protein (S-type) encoded by leek yellow stripe virus (LYSV) isolates detected in Honshu and southward is shorter than the P1 (N-type) of LYSV isolates from garlic grown in Hokkaido due to a large deletion in the N-terminal half. In garlic fields in Hokkaido, two types of LYSV isolate with N- and S-type P1s are sometimes found in mixed infections. In this study, we confirmed that N- and S-type P1 sequences were present in the same plant and that they belong to different evolutionary phylogenetic groups. To investigate how LYSV with S-type P1 (LYSV-S) could have invaded LYSV with N-type P1 (LYSV-N)-infected garlic, we examined wild Allium spp. plants in Hokkaido and found that LYSV was almost undetectable. On the other hand, in Honshu, LYSV-S was detected at a high frequency in Allium spp. other than garlic, suggesting that the LYSV-S can infect a wider host range of Allium spp. compared to LYSV-N. Because P1 proteins of potyviruses have been reported to promote RNA silencing suppressor (RSS) activity of HC-Pro proteins, we analyzed whether the same was true for P1 of LYSV. In onion, contrary to expectation, the P1 protein itself had RSS activity. Moreover, the RSS activity of S-type P1 was considerably stronger than that of N-type P1, suggesting that LYSV P1 may be able to enhance its RSS activity when the deletion is in the N-terminal half and that acquiring S-type P1 may have enabled LYSV to expand its host range.     

CaMKII T286 phosphorylation has distinct essential functions in three forms of long-term plasticity

The Ca²⁺/calmodulin-dependent protein kinase II (CaMKII) mediates long-term potentiation or depression (LTP or LTD) after distinct stimuli of hippocampal NMDA-type glutamate receptors (NMDARs). NMDAR-dependent LTD prevails in juvenile mice, but a mechanistically different form of LTD can be readily induced in adults by instead stimulating metabotropic glutamate receptors (mGluRs). However, the role that CaMKII plays in the mGluR-dependent form of LTD is not clear. Here we show that mGluR-dependent LTD also requires CaMKII and its T286 autophosphorylation (pT286), which induces Ca²⁺-independent autonomous kinase activity. In addition, we compared the role of pT286 among three forms of long-term plasticity (NMDAR-dependent LTP and LTD, and mGluR-dependent LTD) using simultaneous live imaging of endogenous CaMKII together with synaptic marker proteins. We determined that after LTP stimuli, pT286 autophosphorylation accelerated CaMKII movement to excitatory synapses. After NMDAR-LTD stimuli, pT286 was strictly required for any movement to inhibitory synapses. Similar to NMDAR-LTD, we found the mGluR-LTD stimuli did not induce CaMKII movement to excitatory synapses. However, in contrast to NMDAR-LTD, we demonstrate that the mGluR-LTD did not involve CaMKII movement to inhibitory synapses and did not require additional T305/306 autophosphorylation. Thus, despite its prominent role in LTP, we conclude that CaMKII T286 autophosphorylation is also required for both major forms of hippocampal LTD, albeit with differential requirements for the heterosynaptic communication of excitatory signals to inhibitory synapses.