棉花枯萎、黄萎病拮抗芽孢杆菌的抗菌蛋白特性

从土贝母和腊肠等中药和发酵食品中筛选出对棉花枯萎、黄萎病菌有广谱拮抗作用的芽孢杆菌29株,其中有12株菌产抗菌蛋白。有5株抑菌活性较强:H110、H184、H216、B316和B382。经初步鉴定,H110和H184为枯草芽孢杆菌,H216、B316和B382为地衣芽孢杆菌。5株菌的蛋白粗提液对热稳定,对蛋白酶K、胰蛋白酶均不敏感,但H184、H216的蛋白粗提液对胃蛋白酶部分敏感。     

水稻内生枯草芽孢杆菌G87抗菌蛋白的分离纯化及理化特性

【目的】为得到枯草芽孢杆菌(Bacillus subtilis)G87的抗菌蛋白,明确其蛋白理化特性。【方法】采用硫酸铵沉淀和柱层析法进行分离纯化。【结果】获得单一抗菌活性蛋白(峰6-2-1),此抗菌蛋白分子量为50.8 kDa,等电点为5.90。经初步分析,抗菌蛋白不含脂,而含有少量(0.62%)糖;其蛋白部分具有脯氨酸或羟脯氨酸,但不含芳香族氨基酸。抗菌蛋白在高温(≥60℃)和较碱(pH8)环境下活性明显下降,但较抗紫外线、氯仿和胰蛋白酶、蛋白酶K、胃蛋白酶。【结论】枯草芽孢杆菌G87的抗菌蛋白为不含芳烃的糖蛋白,对高温和碱性条件敏感,而对蛋白酶类和紫外线等不敏感。     

蛇毒抗菌的比较性研究

目的 研究蛇毒粗毒的抗菌作用,并比较不同蛇毒对不同细菌的抑制效果.方法 采用抑菌环法测定蛇岛蝮、江浙蝮和短尾蝮蛇毒粗毒对金黄色葡萄球菌、枯草芽孢杆菌、大肠埃希菌、铜绿假单胞菌以及白色念珠菌的抗菌作用,比较不同蛇毒粗毒的抗菌效果;加入过氧化氢酶(catalase),考察蛇毒抗菌作用的变化.结果 (1)3种蛇毒粗毒对5种细菌均呈现不同程度的抑制作用.(2)3种蛇毒粗毒对5种细菌的抑制作用大小依次为:金黄色葡萄球菌＞白色念珠菌＞大肠埃希菌或铜绿假单胞菌＞枯草芽孢杆菌.(3)加入catalase后,蛇毒的抗菌作用明显减弱.结论 (1)3种蛇毒粗毒均具有一定的抗菌作用,并具有明显抑菌选择性.(2)3种蛇毒的抗菌效果不同,蛇岛蝮蛇抗菌作用最强.(3) catalase能显著降低蛇毒的抗菌活性,表明L-氨基酸氧化酶是蛇毒起抗菌作用的主要成分.     

地衣芽孢杆菌W10菌液和抗菌蛋白对桃果实贮藏保鲜效果的影响

以桃‘沪油018’(Amygdalus persica ‘Huyou 018’)果实为试验材料,经地衣芽孢杆菌W10菌液及其抗菌蛋白浸果后常温条件下(25 ℃)贮藏,定期测量桃果各项保鲜指标。结果表明,与对照桃果实比较,地衣芽孢杆菌W10菌液和抗菌蛋白处理可提高桃果实色泽、硬度和可溶性固形物含量,显著降低桃果失重率和腐烂率。经菌液处理桃果腐烂率降低至20%,菌液抑制桃果腐烂效果与多菌灵类似。菌液和抗菌蛋白在提高贮藏期桃果品质方面差异不显著。地衣芽孢杆菌W10菌液和抗菌蛋白应用于采后桃果的贮藏保鲜效果较好,潜力较大。     

抗菌蛋白产生菌TG26的筛选及其培养条件

从丝瓜(Luffa cylindrica(L.)Roem.)根部分离纯化并筛选出强烈抑制小麦赤霉病菌(Gibberella zeae)生长、产大量抗菌蛋白的芽孢杆菌(Bacillus spp.)TG26菌株。用异步培养法检测了该菌株的抗菌活性,比对照菌株 B.subtilis A014和 B_(?)的活性强;平板扩散法测定的 TG26抗菌谱表明,该菌株除抑制小麦赤霉病菌外,对烟草赤星病菌(Alternaria longipes)、棉花枯萎病菌(F.oxysporum f.vasinfectum)、西瓜枯萎病菌(F.oxysporum f.niveum)和绿色木霉(Trichoderma viride)等植物病原真菌以及烟草青枯病菌(Psendomonassolanaceanum)和水稻白叶枯病菌(Xanthomonas campestris pv.oryzae)等植物病原细菌均表现出很强的拮抗作用。TG26菌株产抗菌蛋白的最适培养条件为:选用 BPY 液体培养基,起始 pH7.0。接种后30℃振荡培养36小时的培养液经70%饱合度(NH_4)_2SO_4盐析得到130 mg/L 以上的粗蛋白。该蛋白对温度不敏感,对蛋白酶 K 部分敏感。     

枯草芽孢杆菌TF26抗菌蛋白抑菌活性的初步研究

目的:研究枯草芽孢杆菌TF26抗菌蛋白的抑菌活性和生物稳定性,为菌株及抗菌蛋白的应用提供理论依据.方法:采用硫酸铵盐析方法提取抗菌蛋白,采用菌丝生长速率法检测其对13种植物病原真菌的抑菌活性,采用抑菌圈方法对其生物稳定性进行分析.结果:抗菌蛋白粗提物能够抑制13种植物病原真菌的生长,平皿抑制率为74.3％ ～91.3％,对葵花菌核病菌、番茄和黄瓜枯萎病菌、黄瓜菌核病菌和立枯病菌、水稻恶苗病菌和大豆根腐病菌抑制作用较强.抗菌蛋白在100℃以下,pH＜ 10范围内抑菌活性稳定,对紫外线照射不敏感,室温(20℃)和4℃储存150d抑菌活性稳定.结论:抗菌蛋白具有较强的热、酸碱、紫外和储存稳定性以及广谱的抑菌活性.     

柚皮果胶水解物的抗菌活性研究

以果胶酶为催化剂对柚皮果胶进行了水解,得到不同果胶水解物,探讨水解时间对其抑菌活性的影响;采用两倍稀释法测定了适宜水解的柚皮果胶对大肠杆菌、枯草芽孢杆菌和金黄色葡萄球菌的抗菌作用。结果表明,适度水解的柚皮果胶具有明显的抗菌作用,其对大肠杆菌、枯草芽孢杆菌和金黄色葡萄球菌的最低抑菌质量浓度分别为3.75、7.50和3.75 g.L-1,最低杀菌质量浓度分别为3.75、7.50和7.50 g.L-1。     

家蝇幼虫抗菌相关蛋白/多肽的诱导及抗菌活性分析

对家蝇Musca domestica 3龄幼虫进行针刺、带菌针刺、热激和超声4种处理,并于处理后不同时间分别收集提取家蝇幼虫体内耐热总蛋白,比浊法测定其抗菌活性,经逐步回归分析确定抗菌相关蛋白/多肽。结果表明,4种处理均能诱导家蝇幼虫产生抗菌物质,其中表观分子量为22 kD的蛋白对藤黄微球菌和大肠杆菌均有抗菌作用,50 kD,13 kD,26 kD,7 kD的蛋白抗菌活性具有专一性。还发现一种37 kD的蛋白对抗菌活性有负作用,推测它可能是促进细胞生长的物质。     

白星花金龟(Protaetia brevitarsis)幼虫抗菌物质的分离纯化

以药用昆虫白星花金龟(Protaetia brevitarsis)幼虫为研究对象,通过Sephadex G-50、RP-HPLC等技术分离纯化天然抗菌活性物质.经初步鉴定,该系列抗菌活性物质对枯草芽孢杆菌(Bacillus subttilis)表现出较强的抑菌活性.用MALDI-TOF MS对样品进行分析,检测到相对分子质量分别为2254.045 9、2622.4438的两种抗菌活性物质.推测这些抗菌活性物质在白星花金龟幼虫抵御微生物的侵袭中起到重要作用.     

中蜂抗菌物质的诱导

本文报道了用大肠杆菌注射处理中蜂Ａｐｉｓ ｃｅｒａｎａ Ｆａｂｒｉｃｉｕｓ后,用含菌培养基平板测活法,就中蜂抗菌物质的产生规律及抗菌活性进行了初步研究。结果表明,不同诱导源均可诱导中蜂产生抗菌物质,但诱导的抗菌物质的抗菌活性则有一定的差异。用大肠杆菌重复诱导则使中蜂的成活率和抗菌物质的抗菌活性有很大提高。注射大肠杆菌后冲蜂抗菌物持产生高峰在４８小时左右。诱导后产生的抗菌物质具有广谱性,对大肠杆菌Ａｓｃｈｅｒｉｃｈｉａ　ｃｏｌｉ、枯草芽孢杆菌 Ｂａｃｉｌｌｕｓ　 ｓｕｂｔｉｌｉｓ、苏云金杆菌 Ｂａｃｉｌｌｕｓ　ｔｈｕｒｉｎｇ－ｉｅｎｓｉｓ、巨大芽孢杆菌 Ｂａｃｉｌｌｕｓ　ｍｅｇａｔｈｅｒｉｕｍ、黑腐菌 Ｘａｎｔｈｏｍｏｎａｓ ｃａｍｐｅｓｔｒｉｓ　等均有抑菌作用,而对真菌白僵菌Ｂｅａｕｖｅｒｉａ　ｂａｓｓｉａｎａ未发现抑菌作用。中蜂麻醉方法以冷冻法最为简便、易行。     

Gonadotropin-releasing hormone binding inhibitors in the ovary

A protein present in ovaries and other tissues of many species competitively and reversibly inhibits high affinity binding of gonadotropin-releasing hormone (GnRH) to rat ovarian membranes, but this protein is not GnRH. This protein has been partially purified and characterized from bovine ovaries. The absence of GnRH binding inhibitory (GBI) activity in plasma and follicular fluid indicates that this protein may act in a localized manner within or near its site of production or release. The bovine ovarian GBI protein evokes antigonadotropic activity in ovarian cells from both the rat and the bovine. The biological effect of GBI may occur independently of interaction with high affinity binding sites for GnRH, since these are absent from the bovine ovary. Thus, the GBI protein may abrogate gonadotropin-dependent responses in ovarian cells by mechanisms separate from interaction with GnRH receptors. A complete characterization of the GBI protein and evaluation of its mechanism of action in ovarian and pituitary cells will dictate conclusions on the physiological importance of this protein.     

Altered properties of cAMP-dependent protein kinase in H-ras-transformed NIH3T3 cells

cAMP-dependent protein kinase activity in the soluble fraction was decreased in both v-H-ras-transformed and activated-c-H-ras-transformed NIH3T3 cells as compared with that in NIH3T3 cells. Both of the elution profile of type II cAMP-dependent protein kinase from DEAE-cellulose and the electrophoretic behavior of its regulatory subunits in the particulate fraction of H-ras-transformed cells are different from those of control NIH3T3 cells. These results suggest that ras protein causes the alterations of some properties of cAMP-dependent protein kinases.     

Characterization of an alternate form of Newcastle disease virus fusion protein

The sequence and structure of the Newcastle disease virus (NDV) fusion (F) protein are consistent with its classification as a type 1 glycoprotein. We have previously reported, however, that F protein can be detected in at least two topological forms with respect to membranes in both a cell-free protein synthesizing system containing membranes and infected COS-7 cells (J. Virol. 77:1951-1963, 2003). One form is the classical type 1 glycoprotein, while the other is a polytopic form in which approximately 200 amino acids of the amino-terminal end as well as the cytoplasmic domain (CT) are translocated across membranes. Furthermore, we detected CT sequences on surfaces of F protein-expressing cells, and antibodies specific for these sequences inhibited red blood cell fusion to hemagglutinin-neuraminidase and F protein-expressing cells, suggesting a role for surface-expressed CT sequences in cell-cell fusion. Extending these findings, we have found that the alternate form of the F protein can also be detected in infected and transfected avian cells, the natural host cells of NDV. Furthermore, the alternate form of the F protein was also found in virions released from both infected COS-7 cells and avian cells by Western analysis. Mass spectrometry confirmed its presence in virions released from avian cells. Two different polyclonal antibodies raised against sequences of the CT domain of the F protein slowed plaque formation in both avian and COS-7 cells. Antibody specific for the CT domain also inhibited single-cycle infections, as detected by immunofluorescence of viral proteins in infected cells. The potential roles of this alternate form of the NDV F protein in infection are discussed.     

Cadherin-dependent cell morphology in an epithelium: constructing a quantitative dynamical model

Cells in the Drosophila retina have well-defined morphologies that are attained during tissue morphogenesis. We present a computer simulation of the epithelial tissue in which the global interfacial energy between cells is minimized. Experimental data for both normal cells and mutant cells either lacking or misexpressing the adhesion protein N-cadherin can be explained by a simple model incorporating salient features of morphogenesis that include the timing of N-cadherin expression in cells and its temporal relationship to the remodeling of cell-cell contacts. The simulations reproduce the geometries of wild-type and mutant cells, distinguish features of cadherin dynamics, and emphasize the importance of adhesion protein biogenesis and its timing with respect to cell remodeling. The simulations also indicate that N-cadherin protein is recycled from inactive interfaces to active interfaces, thereby modulating adhesion strengths between cells.     

Baculovirus IE2 Stimulates the Expression of Heat Shock Proteins in Insect and Mammalian Cells to Facilitate Its Proper Functioning

Baculoviruses have gained popularity as pest control agents and for protein production in insect systems. These viruses are also becoming popular for gene expression, tissue engineering and gene therapy in mammalian systems. Baculovirus infection triggers a heat shock response, and this response is crucial for its successful infection of host insect cells. However, the viral protein(s) or factor(s) that trigger this response are not yet clear. Previously, we revealed that IE2-an early gene product of the baculovirus-could form unique nuclear bodies for the strong trans-activation of various promoters in mammalian cells. Here, we purified IE2 nuclear bodies from Vero E6 cells and investigated the associated proteins by using mass spectrometry. Heat shock proteins (HSPs) were found to be one of the major IE2-associated proteins. Our experiments show that HSPs are greatly induced by IE2 and are crucial for the trans-activation function of IE2. Interestingly, blocking both heat shock protein expression and the proteasome pathway preserved the IE2 protein and its nuclear body structure, and revived its function. These observations reveal that HSPs do not function directly to assist the formation of the nuclear body structure, but may rather protect IE2 from proteasome degradation. Aside from functional studies in mammalian cells, we also show that HSPs were stimulated and required to determine IE2 protein levels, in insect cells infected with baculovirus. Upon inhibiting the expression of heat shock proteins, baculovirus IE2 was substantially suppressed, resulting in a significantly suppressed viral titer. Thus, we demonstrate a unique feature in that IE2 can function in both insect and non-host mammalian cells to stimulate HSPs, which may be associated with IE2 stabilization and lead to the protection of the its strong gene activation function in mammalian cells. On the other hand, during viral infection in insect cells, IE2 could also strongly stimulate HSPs and ultimately affect viral replication.     

Primary structure of human protein pS2

We have previously reported that pS2 mRNA expressed in cultured epithelial cells derived from a hormone-dependent breast carcinoma (MCF-7 cells) is also expressed in mucosa cells of normal human stomach. This mRNA encodes a putative 84 amino-acid-long protein, which is secreted by both cell types after elimination of a signal peptide. We report here the purification of the pS2 protein, its trypsin digestion and amino-acid sequencing. The MCF-7 cell-secreted protein is 60 amino-acid-long and its sequence is in complete agreement with that deduced from the mRNA sequence. The presence of an N-terminal glutamic acid indicates that the signal peptidase releases a 24 amino-acid-long signal peptide. Analysis of tryptic peptides derived from the secreted gastric pS2 protein indicates that the signal peptide and the sequence of the first 48 amino-acids are identical to those of secreted MCF-7 pS2 protein, although the N-terminal amino-acid of the gastric protein may be cyclized as a pyroglumatic acid.     

Immunohistochemical localization of plasma retinolbinding protein and prealbumin in human pancreatic islets

Summary This study was undertaken, employing the immunoenzyme method, to confirm the presence of retinol-binding protein in human pancreatic islets, and to compare its distribution with that of prealbumin, insulin, glucagon, somatostatin and pancreatic polypeptide. It was found that most islet cells contained retinol-binding protein, although centrally located cells showed stronger reactivity than those in the peripheral region. The distribution of each of the five polypeptides differed from that of retinolbinding protein, indicating that these peptides did not cross-react with anti-retinol-binding protein antibody. Islet cells which contained prealbumin, on the other hand, were mostly classified as A cells. Further studies are necessary to confirm whether the islet cells produce retinol-binding protein or only store it.     

The unique amino-terminal region of the PDE4D5 cAMP phosphodiesterase isoform confers preferential interaction with beta-arrestins

Isoproterenol challenge of Hek-B2 cells causes a transient recruitment of the endogenous PDE4D isoforms found in these cells, namely PDE4D3 and PDE4D5, to the membrane fraction. PDE4D5 provides around 80% of the total PDE4D protein so recruited, although it only comprises about 40% of the total PDE4D protein in Hek-B2 cells. PDE4D5 provides about 80% of the total PDE4D protein found associated with beta-arrestins immunopurified from Hek-B2, COS1, and A549 cells as well as cardiac myocytes, whereas its overall level in these cells is between 15 and 50% of the total PDE4D protein. Truncation analyses indicate that two sites in PDE4D5 are involved in mediating its interaction with beta-arrestins, one associated with the common PDE4 catalytic region and the other located within its unique amino-terminal region. Truncation analyses indicate that two sites in beta-arrestin 2 are involved in mediating its interaction with PDE4D5, one associated with its extreme amino-terminal region and the other located within the carboxyl-terminal domain of the protein. We suggest that the unique amino-terminal region of PDE4D5 allows it to preferentially interact with beta-arrestins. This specificity appears likely to account for the preferential recruitment of PDE4D5, compared with PDE4D3, to membranes of Hek-B2 cells and cardiac myocytes upon challenge with isoproterenol.