粗糙脉孢菌转录因子LAH-3参与渗透压调控

【目的】通过构建转录因子lah-3基因缺失突变体,研究lah-3基因缺失突变体菌株的渗透压表型,进而探究lah-3基因在渗透压调控中的作用。【方法】采用同源基因重组敲除技术构建lah-3基因缺失突变体。用4%NaCl和1 mol/L Sorbitol进行渗透压处理。利用Northern blot检测渗透压应答基因的表达。利用Westhern blot检测LAH-3蛋白磷酸化修饰水平,OS-2蛋白的表达水平及其磷酸化修饰水平。【结果】在转录因子lah-3基因缺失突变体中,渗透压应答基因gcy-1、stl-1以及pck-1的表达水平都明显降低,而且在渗透压刺激下,LAH-3蛋白磷酸化修饰水平升高。LAH-3的磷酸化修饰不受OS-2调控。lah-3基因的缺失既不影响OS-2蛋白的表达水平,也不影响其在渗透压刺激后的磷酸化修饰。【结论】粗糙脉孢菌中转录因子LAH-3参与调控渗透压应答基因的转录,但其响应过程不依赖于OS-2 MAPK信号通路。     

氯霉素处理对拟南芥STN7和STN8基因表达的影响

本实验运用多肽抗体、磷酸化抗体和半定量RT-PCR技术,研究了叶绿体蛋白合成抑制剂--氯霉素(CAP)处理对拟南芥叶片在生长光强下LHCⅡ蛋白与PSⅡ核心蛋白的磷酸化、STN7和STN8基因在mRNA水平和蛋白水平的变化.结果显示:与对照相比,CAP处理叶片在生长光强下STN7基因表达的mRNA水平减少,类囊体膜上酶蛋白含量较低,LHCⅡ蛋白磷酸化水平也较低;而STN8基因表达的mRNA水平增加,类囊体膜上酶蛋白含量增加了1倍,与PSⅡ核心蛋白中D1、D2和CP43的磷酸化水平较高相吻合.研究表明,氯霉素抑制叶绿体蛋白合成后并影响核基因STN7和STN8的表达.     

拟南芥不同组织基因表达及可变剪接差异分析

可变剪接是转录后重要的基因表达调控方式,也是转录组和蛋白质组多样性的重要来源. 近年来随着拟南芥、水稻、玉米等植物转录组测序的完成,研究人员发现植物pre-mRNA可变剪接的发生与组织分化、发育等生物学过程密切相关. 本工作基于GEO数据库的RNA-seq数据,使用高通量测序数据分析常用的Trimmomatic、Salmon、DESeq2、SUPPA2等工具,识别了拟南芥的种子、根、叶、花、花梗、节间、长角果共7种组织的表达基因和可变剪接事件,以及7种组织间的差异表达基因和差异可变剪接事件,并以叶和花为例展示了相应的生物学功能分析. 该工作系统地研究了拟南芥基因表达和可变剪接发生的组织特异性,有助于进一步阐明植物基因组的基因表达调控机制.     

番茄乙烯信号转录因子LeERF2多克隆抗体的制备

目的:作为番茄乙烯信号转录因子,LeERF2是在蛋白水平单独或同其他蛋白质协同与启动子或增强子相结合发挥其调控功能的,蛋白质的调控机制是信号转导领域中的关键研究内容。本研究目的是制备LeERF2抗体用于探讨番茄乙烯信号转录因子LeERF2在蛋白水平的生物活性及其生物学功能。方法:通过免疫新西兰大耳白雄兔和DEAE-52离子交换柱纯化分离制备了抗LeERF2多克隆抗体。结果与结论:抗体的效价大于10000,纯度达到了99%,Western印迹检测纯化后抗LeERF2多克隆抗体具有免疫特异性。     

拟南芥R2R3-MYB家族第22亚族的结构与功能

拟南芥R2R3-MYB转录因子在拟南芥生长发育、代谢及响应生物和非生物胁迫的调控网络中具有重要作用。根据保守的氨基酸序列,R2R3-MYB转录因子被分为25个亚族,其中第22亚族包含AtMYB44、AtMYB77、AtMYB73和AtMYB70 4个基因,主要响应生物和非生物胁迫。文章从基因功能的相似性、基因表达的一致性和基因结构的保守性3方面综述了第22亚族的4个基因,并综合讨论了其在结构与功能上的冗余性和多样性。     

饱和白光引起的光系统Ⅱ捕光复合体（LHCⅡ）从反应中心复合体脱离不同于弱红光引起的状态1向状态2的转换

我们观测了不同光照预处理对拟南芥、小麦和大豆叶片光合作用和低温（77K）叶绿素荧光参数F685、F735和F685／F735的影响。野生型拟南芥叶片光合作用对饱和光到有限光转变的响应曲线是V型,而缺乏叶绿体蛋白激酶的突变体STN7的这一曲线为L型。饱和白光可以引起拟南芥叶片F685／F735的明显降低,但是F735没有明显增高,而弱红光可以导致拟南芥叶片F685／F735的明显降低和F735的明显增高,表明弱红光可以引起状态1向状态2的转变,同时伴随从光系统Ⅱ脱离的LHCⅡ与光系统Ⅰ的结合,而饱和白光只能引起LHCⅡ从光系统Ⅱ反应中心复合体脱离。并且,低温叶绿素荧光分析结果证明,饱和白光可以引起大豆叶片LHCⅡ脱离,但是不能引起小麦叶片LHCⅡ脱离,而弱红光可以引起小麦叶片的这种状态转换,却不能引起大豆叶片的这种状态转换。因此,饱和白光引起的野生型拟南芥和大豆叶片的LHCⅡ脱离不是一个典型的状态转换现象。     

利用四环素调控系统研究 CHIP 对TGF-β信号通路的抑制性调节

为了研究伴侣分子相互作用蛋白 CHIP 对 TGF-β信号通路的调控,利用四环素基因表达调控系统,建立四环素调控表达 CHIP 的稳定细胞系 (Mv1Lu-Tet off-CHIP). 利用此细胞模型,发现 CHIP 的过量表达可显著降低细胞内 Smad2/3 蛋白水平;荧光素酶报告分析也表明开启 CHIP 蛋白表达可明显降低 Smads 介导的基因转录活性;进一步的免疫印迹结果显示 CHIP 蛋白可明显下调 TGF-β所诱导的下游基因 JunB 的表达 . 上述结果提示 CHIP 可以作为一种新的蛋白质分子抑制性调节 TGF-β信号通路 .     

AP-1在AngⅡ正反馈调节其前体基因表达中的作用

血管紧张素Ⅱ(AngⅡ)可诱导其前体基因在血管平滑肌细胞(vascularsmoothmusclecells,VSMC)中进行表达,其作用机制与促进转录激活蛋白-1(activatingprotein-1,AP-1)的基因调控区中存在的AP-1位点结合有关.为进一步明确AngⅡ调节AP-1结合活性的分子机制,用放线菌酮(cycloheximide,CHX)作为c-Jun磷酸化抑制剂,经DNA-蛋白质相互作用和蛋白质印迹实验,探讨AngⅡ对AP-1结合活性的影响并探讨其分子机制.结果表明,受AngⅡ刺激的VSMC,其核蛋白中AP-1的组成亚基之一c-Jun水平明显升高.免疫细胞化学染色显示,在被AngⅡ处理的细胞中,c-Jun主要定位于细胞核,胞浆中几乎检测不出该转录激活蛋白的存在.用丝氨酸磷酸化抗体检测证实,AngⅡ可诱导c-Jun磷酸化.电泳迁移率改变分析(electrophoreticmobilityshiftassay,EMSA)显示,c-Jun的磷酸化水平与AP-1结合血管紧张素原基因顺式元件的活性,和对该基因的转录激活作用呈正相关关系,CHX通过阻断c-Jun磷酸化抑制AngⅡ诱导的AP-1结合活性,但是不影响c-Jun的表达水平.上述结果提示,AP-1的磷酸化活化是AngⅡ正反馈调节其前体基因表达的重要机制之一,首次发现CHX是c-Jun磷酸化的抑制剂.     

谷子MYB-CC基因家族的鉴定与表达分析

MYB-CC基因家族是由MYB-DNA结合域和CC(coiled-coil)结构域组成的,其中CC结构域能通过折叠参与蛋白质之间的相互作用,是一个二聚体结构域.这类MYB-CC转录因子是植物特有的,除磷饥饿响应蛋白1(PHR1)外,拟南芥中另外14个蛋白也同样具有这两个结构域.部分MYB-CC基因已经被证明可调控植物中...     

转录因子网络与植物对环境胁迫的响应

转录因子所介导的基因表达调控网络在植物抵御各种环境胁迫的反应中具有重要功能.已鉴定的参与植物环境胁迫响应的转录因子及家族有APETALA2/EREBP、BZIP、WRKY和MYB等.这些转录因子组成调控网络,精细调控植物胁迫反应中各种相关基因的表达.转录因子及其调控网络的遗传修饰已成为从系统水平上探索胁迫生物学和提高植物胁迫耐性和抗性的有效工具.     

壳聚糖酶的克隆表达与壳寡糖的制备分析

目的:克隆壳聚糖酶基因于大肠杆菌中实现高表达,制备壳寡糖。方法:以枯草芽孢杆菌总DNA为模板扩增壳聚糖酶基因(CSN),克隆至载体pET23a(+)上,转化菌株BL21(DE3)。重组子经0.5 mmol/L IPTG诱导后,SDS-PAGE和质谱检测与鉴定重组酶。酶纯化后水解壳聚糖,薄层色谱分析其水解产物。结果:质谱证明壳聚糖酶(31.5kDa)成功表达,表达量占菌体总蛋白的45%左右。纯化后重组酶浓度为900 mg/L,纯度95%、回收率85%,酶活力为10 000 U/mg。壳聚糖降解产物为壳二糖至壳四糖。结论:原核表达载体pET23a(+)-CSN构建正确,壳聚糖酶表达量与活性高,适用于水解壳聚糖制备壳寡糖。     

国内外蝗害治理技术现状与展望

本文首先概述了国内外蝗虫发生与为害的态势,总结了现阶段我国蝗虫发生与为害的主要特点:即农田飞蝗暴发频繁而且严重,草原土蝗的发生时常造成严重的经济损失,而且侵入城市干扰市民生活,我国与周边国家之间蝗虫过境迁移频繁,使用化学农药污染环境和农产品;分析了国内外蝗虫防治对策与技术的发展现状,重点介绍了应急防治和可持续治理对策、...     

Synthesis and turnover of cerebrosides and phosphatidylserine of myelin and microsomal fractions of adult and developing rat brain.

The synthesis and turnover of cerebrosides and phospholipids was followed in microsomal and myelin fractions of developing and adult rat brains after an intracerebral injection of [U-14C]serine. The kinetics of incorporation of radioactivity into microsomal and myelin cerebrosides indicate the possibility of a precursor-product relationship between cerebrosides of these membranes. The specific radioactivity of myelin cerebrosides was corrected for the deposition of newly formed cerebrosides in myelin. Multiphasic curves were obtained for the decline in specific radioactivity of myelin and microsomal cerebrosides, suggesting different cerebroside pools in these membranes. The half-life of the fast turning-over pool of cerebrosides of myelin was 7 and 22 days for the developing and adult rat brain respectively. The half-life of the slowly turning-over pool of myelin cerebrosides was about 145 days for both groups of animals. The half-life of the rapidly turning-over microsomal cerebrosides was calculated to be 20 and 40 h for the developing and adult animals respectively. The half-life of the intermediate and slowly turning-over microsomal cerebrosides was 11 and 60 days respectively, for both groups of animals. The amount of incorporation of radioactivity into microsomal cerebrosides from L-serine was greatly decreased in the adult animals, and greater amounts of the precursor were directed towards the synthesis of phosphatidylserine. In the developing animals, considerable amounts of cerebrosides were synthesized from L-serine, besides phosphatidylserine. The time-course of incorporation indicated that a precursor-product relationship exists between microsomal and myelin phosphatidylserine. The half-life of microsomal phosphatidylserine was calculated to be about 8 h for the fast turning-over pool in both groups of animals.     

Identification and composition of the tonsillar and anal enterococcal and streptococcal flora of dogs and cats

Enterococcus faecalis was the most frequently isolated enterococcal species from anal swabs and tonsils of dogs and cats, although in the anal samples from dogs Ent. hirae was found almost as often as Ent. faecalis. Most Ent.faecium strains from dog tonsils differed from those associated with humans and other animals in that they fermented sorbitol. Typical Ent. avium as well as atypical Ent. avium -like strains were seen in dogs, while the related species Ent. raffinosus was associated with cat tonsils. Enterococcus cecorum also occurred mainly in cats. Certain atypical strains, presumptively identified as Ent. cecorum , shared characteristics with Ent. columbae.
The most frequent streptococcal species in tonsils of cats and dogs were Streptococcus suis and Strep. canis. Streptococcus canis and Strep. bovis predominated in anal swabs. The canine Strep. suis differed from the common porcine strains in fermenting mannitol.
Forty-seven of the 288 isolates examined could not be identified or related to known species. The characteristics of two groups of these bacteria, provisionally called 'Ton 31 group' and 'O7 group' are described.     

Molecular characterisation of species and genotypes of Cryptosporidium and Giardia and assessment of zoonotic transmission

The molecular characterisation of species and genotypes of Cryptosporidium and Giardia is essential for accurately identifying organisms and assessing zoonotic transmission. Results of recent molecular epidemiological studies strongly suggest that zoonotic transmission plays an important role in cryptosporidiosis epidemiology. In such cases the most prevalent zoonotic species is Cryptosporidium parvum. Genotyping and subtyping data suggest that zoonotic transmission is not as prevalent in the epidemiology of giardiasis. Molecular characterisation of Cryptosporidium and Giardia is a relatively recent application that is evolving as new genes are found that increase the accuracy of identification while discovering a greater diversity of species and yet unnamed taxa within these two important genera. As molecular data accumulate, our understanding of the role of zoonotic transmission in epidemiology and clinical manifestations is becoming clearer.     

白术同源四倍体的诱导和鉴定及其与二倍体过氧化物酶的比较

以白术（Atractylodes macrooephala Koidz.）二倍体组培苗为材料,对其四倍体诱导方法进行研究,共获得45个白术同源四倍体株系,为优良株系的选育提供了材料。此外,还分析比较了其中8个白术四倍体株系与二倍体的过氧化物酶同工酶（POD）的酶谱差异,发现四倍体各株系过氧化物酶同工酶谱比二倍体的均多了Rf0.310的谱带,且总过氧化物酶比活力也发生了很大改变,对探讨白术四倍体优良株系的生理生化机理具有一定的参考价值。     

Kinetics and thermodynamics of peroxidase- and laccase-catalyzed oxidation of N-substituted phenothiazines and phenoxazines

N -substituted phenothiazines (PTs) and phenoxazines (POs) catalyzed by fungal Coprinus cinereus peroxidase and Polyporus pinsitus laccase were investigated at pH 4–10. In the case of peroxidase, an apparent bimolecular rate constant (expressed as k _cat/K _m) varied from 1 ×10⁷M⁻¹s⁻¹to 2.6×10⁸M⁻¹s⁻¹ at pH 7.0. The constants for PO oxidation were higher in comparison to PT. pH dependence revealed two or three ionizable groups with pK _a values of 4.9–5.7 and 7.7–9.7 that significantly affected the activity of peroxidase. Single-turnover experiments showed that the limiting step of PT oxidation was reduction of compound II and second-order rate constants were obtained which were consistent with the constants at steady-state conditions. Laccase-catalyzed PT and PO oxidation rates were lower; apparent bimolecular rate constants varied from 1.8×10⁵M⁻¹s⁻¹ to 2.0×10⁷M⁻¹s⁻¹ at pH 5.3. PO constants were higher in comparison to PT, as was the case with peroxidase. The dependence of the apparent bimolecular constants of compound II or copper type 1 reduction, in the case of peroxidase or laccase, respectively, was analyzed in the framework of the Marcus outer-sphere electron-transfer theory. Peroxidase-catalyzed reactions with PT, as well as PO, fitted the same hyperbolic dependence with a maximal oxidation rate of 1.6×10⁸M⁻¹s⁻¹ and a reorganization energy of 0.30 eV. The respective parameters for laccase were 5.0×10⁷M⁻¹s⁻¹ and 0.29 eV. Received: 20 September 1999 / Accepted: 24 February 2000