产黄酮甘蔗叶内生真菌的分离与鉴定

采用显色反应、薄层层析色谱和紫外吸收光谱法,对甘蔗叶内16株内生真菌的代谢产物进行黄酮类化合物检测。结果共筛选到3株能够产黄酮类化合物的内生真菌(GZ-1、GZ-4和GZ-5)。依据真菌的形态特征及ITS序列分析,鉴定结果表明菌株GZ-1、GZ-5为棘孢曲霉(Aspergillus aculeatus),菌株GZ-4为黑曲霉(Aspergillus niger)。     

从南方红豆杉中筛选和鉴定25株产紫杉烷的内生真菌

为从南方红豆杉(Taxus chinensis var.mairei)中分离产紫杉烷的内生真菌,从其幼茎、树皮和叶片中分离纯化了491株内生真菌,经筛选获得25株内生真菌具有产紫杉烷的能力,其中,4株可产紫杉醇、巴卡亭Ⅲ和10-去乙酰巴卡亭Ⅲ,8株能产紫杉醇和巴卡亭Ⅲ,1株能产紫杉醇和10-去乙酰巴卡亭Ⅲ,1株能产巴卡亭Ⅲ和10-去乙酰巴卡亭Ⅲ,6株仅产紫杉醇,5株仅产巴卡亭Ⅲ。根据内生真菌的来源,幼茎中有11株产紫杉烷的内生真菌,叶片中有9株,而树皮中仅有5株。这些菌株的紫杉醇、巴卡亭和10-去乙酰巴卡亭Ⅲ产量分别为0.64~9.87、0.48~3.42和0.20~1.00μg L~(–1)。因此,南方红豆杉中具有紫杉烷类代谢途径的内生真菌来源广,数量多,是研究真菌中紫杉烷类化合物代谢途径的良好材料,也为紫杉烷类抗癌药生产提供了潜在的真菌种源。     

海南粗榧内生真菌抗肿瘤抗菌活性的筛选

对72株海南粗榧(Cephalotaxus hainanensis Li)内生真菌进行了抗肿瘤和抗菌活性筛选。结果显示, 有9株内生真菌至少对一种指示瘤株具有细胞毒活性, 5株内生真菌对金黄色葡萄球菌有较强的抑菌活性, 1株内生真菌对辣椒疫霉有抑制作用。这表明海南粗榧内生真菌是寻找有价值的生物活性成分的潜在资源, 其生物活性成分值得进一步研究。     

青蒿内生真菌的抗肿瘤抗氧化活性

采用MTT法和DPPH法,分别测定已分离得到的68株贵州青蒿内生真菌乙酸乙酯粗提物的肿瘤细胞生长抑制率和DPPH自由基清除率。试验共筛选获得12株活性内生真菌,根据其形态特征进行鉴定,分别隶属于子囊菌亚门(Ascomycotina)的链格孢属(Alternaria)、刺盘孢属(Colletotrichum)、拟盘多毛孢属(Pestalotiopsis)和拟茎点霉属(Phomopsis);其中,有8株内生真菌至少对1种指示瘤株具有细胞毒活性,占总菌株数的11.8%;5株内生真菌具有不同程度的清除DPPH自由基活性,占总菌株数的7.4%;1株内生真菌同时具有细胞毒活性和抗氧化活性。     

油樟内生真菌产油脂初步研究

采用GC-MS法分析78株油樟内生真菌(其中油樟根内生真菌43株,茎内生真菌11株,叶内生真菌24株)发酵产物,发现半数以上内生真菌能够产C_(16)到C_(19)的脂肪酸及相应的甲酯;利用索氏抽提法提取78株油樟内生真菌的总油脂并采用GC-MS法分析其组分,发现4株内生真菌(编号分别为YG48、YG64、YJ9、YY8)菌丝内油脂相对含量较高,种类较少,其中YG48、YY8几乎只产棕榈酸酯、亚油酸甲酯两种油脂,YG64、YJ9主要产油酸、硬脂酸、棕榈酸甲酯、油酸酰胺及硬脂酰胺。     

产黄芩苷内生真菌的筛选与鉴定

从药用植物黄芩根、茎、叶和花中分离得到17株内生真菌,其发酵液对10种指示菌进行抑菌活性测定,并通过薄层色谱(TLC)和高效液相色谱(HPLC)对所分离到的内生真菌代谢产物进行分析。结果显示,所分离到的内生真菌中12株至少对一种指示菌有抑菌活性,其中3株(G2、J4和J5)具有较广的抑菌作用。从黄芩茎和花中分离得到的2株内生真菌J1、H3可以在人工培养基中产生黄芩活性成分——黄芩苷,结合菌落形态特征、显微观察及ITS序列分析,初步鉴定这2株菌株均属于青霉菌属。     

云南八角莲内生真菌分离、鉴定的初步探索

通过对云南八角莲(D.aurantiocaulis)内生真菌的分离、鉴定,获得87株内生真菌,并对87株进行分离、鉴定发现内生真菌在宿主植物中具有明显的多样性,无孢类群(22株)是优势菌,其次为镰孢菌属(10株)毛壳菌属(10株)、青霉属(9株)、小齿梗霉属(7株)、丛梗孢属(4株),首次报道云南八角莲内生真菌的类群和区系特点.     

黄花夹竹桃内生真菌抗病原细菌的初步研究

从植物黄花夹竹桃 (Thevetiaperuviana)的根、茎、叶、果实中分离出内生真菌 10 1株。以鼠伤寒沙门氏菌 (Salmonellatyphimurium)、肺炎链球菌 (Streptococcuspneumoniae)、乙型溶血链球菌 (Streptococcushemolyticus)、金黄色葡萄球菌 (Staphyllococcusaureus) 4种人类病原菌为指示菌 ,对其进行抑菌活性筛选 ,结果有 17株内生真菌对 1株或 1株以上人类病原菌有抑菌活性 ,其中平板抑菌圈直径大于 2 0mm的菌株有9株。具有抗菌活性的内生真菌分别来自木霉属 (Trichoderma)、曲霉属 (Aspergillus)等 9个属。     

小黄花茶内生真菌的多样性分析及抑菌活性初筛

为探究小黄花茶内生真菌种类和种群分布规律以及对植物病原真菌的抑制作用,该研究采用组织分离法对小黄花茶内生真菌进行分离纯化,基于形态学和分子生物学进行鉴定并结合统计学分析评价其多样性,再通过平板对峙法筛选出具有抑菌活性的菌株。结果表明：(1)从小黄花茶324份组织块中分离得到内生真菌261株,隶属1门5纲9目22属,其中优势属包括炭疽菌属(Colletotrichum)、间座壳属(Diaporthe)、拟盘多毛孢属(Pestalotiopsis),分离频率分别为21.84%、16.86%、10.34%。(2)研究发现小黄花茶内生真菌在不同季节分布不同,冬季分离出的菌株数量最多,为72株(占27.59%,隶属16个属),春季62株(隶属13个属),夏季59株(隶属15个属),秋季68株(隶属13个属),冬季的香农-维纳指数(H′)、辛普森指数(D)、Pielou’s均匀度指数(E)和Margalef’s丰富度指数(M)最高,春季与冬季内生真菌种类相似性较高,夏季与秋季内生真菌种类相似性较高。(3)小黄花茶内生真菌不同部位分布不同,茎中内生真菌的分布最多,有102株(占39.08%,隶属15...     

虎皮楠内生真菌Aspergillus sp.DCS31化学成分研究

从长序虎皮楠韧皮部分离到内生真菌Aspergillus sp.DCS31,经ITS序列分析将该株菌鉴定为曲霉属真菌.我们从该菌的固体发酵物中分离得到了5个化合物,经质谱和核磁共振波谱解析,分别鉴定为asperpyroneD(1)、asperpyrone A(2)、flavasperone(3)、1,2-benzenedicarboxylic acid bis(2α-methyl heptyl)ester (4)、2,5-di-hydroxyphenylacetic acid methyl ester(5).化合物1、2、3、4为首次从虎皮楠内生真菌中分离得到.     

玉米茎基腐病生防菌的筛选及应用

【目的】拟针对禾谷镰孢进行生防菌的筛选和应用研究,以期为玉米茎基腐病生防菌剂的研制奠定基础。【方法】通过对峙培养法对玉米茎基腐病的主要致病菌禾谷镰孢进行玉米内生生防细菌的筛选,从玉米主栽品种九单48幼苗内部获得一株具有较强抑菌效果的内生生防细菌(简称48SJ7-1);基于传统鉴定、16S rRNA基因序列测定及系统发育分析,对48SJ7-1进行鉴定;并通过盆栽试验测定该生防菌株的防效。【结果】菌株48SJ7-1经鉴定为甲基营养型芽孢杆菌,GenBank登录号为KU377993,48SJ7-1盆栽防效为68.47%,与对照药剂2%戊唑醇悬浮种衣剂差异不显著。【结论】48SJ7-1对玉米茎基腐病的主要致病菌禾谷镰孢有较好防效,对玉米生长还有明显的促进作用,而且表观上无药害发生。     

MNB/DYRK1A phosphorylation regulates the interactions of synaptojanin 1 with endocytic accessory proteins

MNB/DYRK1A is a proline-directed serine/threonine kinase implicated in Down syndrome (DS). In an earlier screening, two proteins from adult rat brain, one 100kDa and the other 140 kDa, were found to be prominently phosphorylated by the kinase. The 100-kDa protein was previously characterized as an isoform of dynamin 1. In this study, we identified the 140-kDa protein as synaptojanin 1 (SJ1). MNB/DYRK1A phosphorylates SJ1 at multiple sites and produces complex behaviors in binding to amphiphysin 1 and intersectin 1 (ITSN1). However, the phosphorylation has little effect on the phosphatidylinositol phosphatase activity of SJ1. These results suggest that MNB/DYRK1A is involved in regulating the recruitment activity but not the phosphatase activity of SJ1. Our findings may be especially important in the etiology of DS because MNB/DYRK1A, SJ1, and ITSN1 are all located at or near the region of human chromosome 21, which is postulated to be involved in the disease.     

嗜盐古菌Haloferax sp. D1227中超氧化物歧化酶功能鉴定及其增强细菌耐盐性的研究

【背景】细菌、酵母或植物来源的超氧化物歧化酶(Superoxide dismutase,SOD)编码基因在异源宿主中表达并提高宿主耐盐性的研究已有一些报道,其异源宿主也多为植物,而古菌来源的超氧化物歧化酶编码基因在细菌中成功表达并提高其耐盐性的研究尚无报道。【目的】寻找嗜盐古菌Haloferax sp.D1227中的超氧化物歧化酶编码基因并鉴定其功能,将其在4-硝基苯酚降解细菌Burkholderia sp.SJ98中表达,研究该古菌的超氧化物歧化酶对菌株SJ98耐盐性和降解4-硝基苯酚功能的影响。【方法】通过生物信息学方法寻找嗜盐古菌D1227中潜在的超氧化物歧化酶编码基因,利用表达载体p ET-28a和广泛宿主载体p BBR1MCS-2将其分别在E.coli BL21(DE3)和4-硝基苯酚的降解菌株SJ98中异源表达,检测细胞抽提液和纯化蛋白的超氧化物歧化酶比活力。分别以葡萄糖和4-硝基苯酚为碳源,在M9培养基和添加500 mmol/L Na Cl(Na Cl含量约3%)的M9培养基中分别培养细菌SJ98的重组菌株和空载体重组菌株,利用全自动生长曲线分析仪和高效液相色谱等方法检测重组菌株的生长能力和对4-硝基苯酚的降解能力。【结果】通过生物信息学分析,在嗜盐古菌D1227基因组中发现了潜在的超氧化物歧化酶编码基因sod A,其在E.coli BL21(DE3)和菌株SJ98中分别异源表达均具有超氧化物歧化酶活力[细胞抽提液的比活力分别为21.07±0.02 U/mg和84.56±0.16 U/mg,从BL21(DE3)菌株纯化的蛋白Sod AD1227比活力为179.46±3.43 U/mg]。在添加500 mmol/L Na Cl的M9培养基中培养时,以葡萄糖为碳源,重组菌株SJ98[p BBR-sod A]仍可正常生长,而空载体对照菌株SJ98[p BBR1MCS-2]几乎丧失了生长能力;以4-硝基苯酚为碳源,菌株SJ98[p BBR-sod A]保持了利用底物生长和降解底物的能力,而菌株SJ98[p BBR1MCS-2]的生长和降解能力几乎丧失。用软件Phyre2模拟分析Sod AD1227的单体结构,该蛋白拥有Fe/Mn-SOD家族的典型结构特征,推测其属于Fe/Mn-SOD家族。【结论】本研究为利用古菌SOD对细菌进行改造以适应高盐环境中降解有机污染物的应用提供了潜在的可行性。     

Gliotactin,a novel marker of tricellular junctions,is necessary for septate junction development in Drosophila

Septate junctions (SJs), similar to tight junctions, function as transepithelial permeability barriers. Gliotactin (Gli) is a cholinesterase-like molecule that is necessary for blood-nerve barrier integrity, and may, therefore, contribute to SJ development or function. To address this hypothesis, we analyzed Gli expression and the Gli mutant phenotype in Drosophila epithelia. In Gli mutants, localization of SJ markers neurexin-IV, discs large, and coracle are disrupted. Furthermore, SJ barrier function is lost as determined by dye permeability assays. These data suggest that Gli is necessary for SJ formation. Surprisingly, Gli distribution only colocalizes with other SJ markers at tricellular junctions, suggesting that Gli has a unique function in SJ development. Ultrastructural analysis of Gli mutants supports this notion. In contrast to other SJ mutants in which septa are missing, septa are present in Gli mutants, but the junction has an immature morphology. We propose a model, whereby Gli acts at tricellular junctions to bind, anchor, or compact SJ strands apically during SJ development.     

Slow motile mutant in Salmonella typhimurium

Enomoto, Masatoshi (National Institute of Genetics, Misima, Japan). Slow motile mutant in Salmonella typhimurium. J. Bacteriol. 90:1696-1702. 1965.-A slow motile mutant, SJ399, was isolated from a wild-type strain of Salmonella typhimurium TM2. The mutant was as motile as the wild type in broth culture at 37 C. However, on semisolid medium it produced a much narrower swarming band than TM2. The motility of this mutant was hindered by the viscosity of semisolid medium. H antigenicity and morphological characters of flagella of the mutant were the same as those of the wild type. The motility phage, chi, responded differently to SJ399 and the wild type. Plaques of SJ399 were small and cloudy, whereas on the wild type they were large and clear. The efficiency of plating on SJ399 was 0.36 as compared with 1 with the wild type. Stained preparations revealed that the mutant had about one-third the number of flagella of the wild type. The reduction of the number of flagella also was ascertained by biochemical measurement of flagellar protein which was purified after deflagellation from cells. The content of flagellin in SJ399 was about 32% of that of the wild type. Phage P22-mediated transductions from SJ399 to nonflagellated (fla(-)) and paralyzed (mot(-)) mutants showed that the mutant SJ399 complements seven fla(-) and three mot(-) strains which are representative mutants of flagellation and motility cistrons, respectively. The mutation site of SJ399 was cotransduced with both motA and B cistrons. The two point cross tests between SJ399 and mot mutants revealed that the mutation site of SJ399 is located in the motB cistron. The insertion of the genetic region containing the mutation site of SJ399 to the motB cistron is discussed in relation to intracistronic complementation.     

Direct interaction of the 170 kDa isoform of synaptojanin 1 with clathrin and with the clathrin adaptor AP-2

Synaptojanin 1, a polyphosphoinositide phosphatase, is expressed as two major alternatively spliced isoforms of 145 kDa (SJ145) and 170 kDa (SJ170) [1] [2], which are thought to have pleiotropic roles in endocytosis, signaling and actin function [3] [4] [5]. SJ145 is highly enriched in nerve terminals where it participates in clathrin-dependent synaptic vesicle recycling [1] [5]. SJ170, which differs from SJ145 by the presence of a carboxy-terminal extension, is the predominant isoform in developing neurons and is expressed in a variety of tissues [2]. The carboxy-terminal domain unique to SJ170 was previously shown to bind Eps15 [6], a protein involved in receptor-mediated endocytosis. Here, we show that the same domain also binds clathrin and the clathrin adaptor AP-2. These interactions occur both in vitro and in vivo and are direct. Binding of AP-2 is mediated by the ear domain of its alpha-adaptin subunit and binding of clathrin by the amino-terminal domain of its heavy chain. Overexpression in chinese hamster ovary (CHO) cells of full-length SJ170 or its unique carboxy-terminal region caused mislocalization of Eps15, AP-2 and clathrin, as well as inhibition of clathrin-dependent transferrin uptake. These findings suggest a close association of SJ170 with the clathrin coat and provide new evidence for its physiological role in the regulation of clathrin coat dynamics.     

Identification of intrinsic sialidase and sialoglycoprotein substrates in rat brain synaptic junctions

Sialidase activity associated with rat brain synaptic junctions (SJ) and synaptic membranes (SM) was determined. Both fractions released sialic acid from exogenous glycopeptides and gangliosides. SJ accounted for 5-10% of the total sialidase activity recovered from SM following extraction with Triton X-100, and the specific activity of SJ sialidase was 60% of that of the parent SM fraction. Intrinsic SJ sialidase hydrolysed 12-15% of the sialic acid associated with endogenous SJ glycoproteins. Sialic acid residues associated with SJ glycoproteins were labelled with sodium borotritide and SJ proteins fractionated by affinity chromatography on concanavalin A-agarose. SJ glycoproteins that reacted with concanavalin A (con A+ glycoproteins) accounted for 25% of the total SJ [3H]sialic acid. Intrinsic SJ sialidase hydrolysed 20% of the [3H]sialic acid associated with these glycoproteins. Each molecular weight class of con A+ glycoprotein previously shown to be a specific component of the postsynaptic apparatus contained sialic acid and was acted on by intrinsic SJ sialidase.     

Evidence for phosphatase activity of p27SJ and its impact on the cell cycle

p27SJ, a novel protein isolated from St John's wort (Hypericum perforatum), belongs to an emerging family of DING proteins that are related to a prokaryotic phosphate‐binding protein superfamily. Here we demonstrate that p27SJ exhibits phosphatase activity and that its expression in cells decreases the level of phosphorylated Erk1/2, a key protein of several signaling pathways. Treatment of p27SJ‐expressing cells with phosphatase inhibitors including okadaic acid, maintained Erk1/2 in its phosphorylated form, suggesting that dephosphorylation of Erk1/2 is mediated by p27SJ. Further, expression of p27SJ affects Erk1/2 downstream regulatory targets such as STAT3 and CREB. Moreover, the level of expression of cyclin A that associates with active ERK1/2 and is regulated by CREB, was modestly reduced in p27SJ‐expressing cells. Accordingly, results from in vitro kinase assays revealed a noticeable decrease in the activity of cyclin A in cells expressing p27SJ. Cell cycle analysis demonstrated dysregulation at S and G2/M phases in cells expressing p27SJ, supporting the notion that a decline in cyclin A activity by p27SJ has a biological impact on cell growth. These observations provide evidence that p27SJ alters the state of Erk1/2 phosphorylation, and impacts several biological events associated with cell growth and function. J. Cell. Biochem. 107: 400–407, 2009. © 2009 Wiley‐Liss, Inc.     

Cyclic AMP-stimulated protein kinases at brain synaptic junctions.

We have examined endogenous cyclic AMP-stimulated phosphorylation of subcellular fractions of rat brain enriched in synaptic plasma membranes (SPM), purified synaptic junctions (SJ), and postsynaptic densities (PSD). The analyses of these fractions are essential to provide direct evidence for cyclic AMP-dependent endogenous phosphorylation at discrete synaptic junctional loci. Protein kinase activity was measured in subcellular fractions using both endogenous and exogenous (histones) proteins as substrates. The SJ fraction possessed the highest kinase activity toward endogenous protein substrates, 5-fold greater than SPM and approximately 120-fold greater than PSD fractions. Although the kinase activity as measured with histones as substrates was only slightly higher in SJ than SPM fractions, there was a marked preference of kinase activity toward endogenous compared to exogenous substrates in SJ fractions but in SPM fractions. Although overall phosphorylation in SJ fractions was increased only 36% by 5 micron cyclic AMP, there were discrete proteins of Mr = 85,000, 82,000, 78,000, and 55,000 which incorporated 2- to 3-fold more radioactive phosphate in the presence of cyclic AMP. Most, if not all, of the cyclic AMP-independent kinase activity is probably catalyzed by catalytic subunit derived from cyclic AMP-dependent kinase, since the phosphorylation of both exogenous and endogenous proteins was greatly decreased in the presence of a heat-stable inhibitor protein prepared from the soluble fraction of rat brain. The specific retention of SJ protein kinase(s) activity during purification and their resistance to detergent solubilization was achieved by chemical treatments which produce interprotein cross-linking via disulfide bridges. Two SJ polypeptides of Mr = 55,000 and 49,000 were photoaffinity-labeled with [32P]8-N3-cyclic AMP and probably represent the regulatory subunits of the type I and II cyclic AMP-dependent protein kinases. The protein of Mr = 55,000 was phosphorylated in a cyclic AMP-stimulated manner suggesting autophosphorylation as previously observed in other systems.