壳聚糖对大肠杆菌的抑制作用规律及抗菌机理初探

考察了不同分子量壳聚糖对大肠杆菌的抑菌性能,利用壳聚糖的席夫碱反应对其氨基加以保护,探讨了壳聚糖对大肠杆菌的抗菌机理。研究结果表明:壳聚糖分子量越小,对大肠杆菌的抗菌作用越明显;壳聚糖对大肠杆菌的抑菌作用与其氨基的质子化有关。     

油松毛虫幼虫抗菌物质及其抗菌活性研究

采用体内注射法,对油松毛虫Dendrolimus tabulaeformis Tsai et Liu 3龄幼虫注射浓度为1．0×10^8孢子／mL的大肠杆菌Escherichia coli菌悬液,诱导其产生抗菌物质,12h后收集制备血淋巴粗提液。分别测定对4种细菌和4种真菌的抗菌活性,并检测温度、pH值变化和反复冻融对抗菌活性的影响。采用Tricine—SDS—PAGE电泳法确定抗菌物质的分子量大小。结果发现,诱导后的油松毛虫3龄幼虫血淋巴粗提液对试验的细菌和真菌均有不同程度的抑制作用,其中对革兰氏阴性细菌大肠杆菌E．coli和变形杆菌Proteus species的抑制作用强于革兰氏阳性细菌金黄色葡萄球菌Staphylococcus aureus和枯草芽孢杆菌Bacillus subtilis。血淋巴粗提液的的抗菌活性在50℃水浴处理和4～9的pH值条件下保持稳定,反复冻融1～5次抗菌物质的活性降低4．3％～14．9％。电泳结果显示,诱导组血淋巴粗提液在23．2kD和15．0kD处分别出现一条特异性条带,在60．4kD处蛋自带变浅。由此推测从油松毛虫幼虫体内诱导产生的抗菌物质分子量可能是23．2kD和15．0kD。     

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。     

拮抗菌TG26的鉴定及其抗菌蛋白BI的纯化和部分特性

从丝瓜根部分离出来的桔抗菌ＴＧ２６,根据形态特征和生理生化特性,鉴定为枯草芽抱杆菌（Ｂａｃｉｌｌｕｓｓｕｂｔｉｌｉｓ）。该菌株能分泌大量的抗菌蛋白,经ＳｅｐｈａｄｅｘＧ－１５０柱和ＦＰＬＣＭｏｎｏＱ柱层析后得到单一组分的抗菌蛋白,命名为ＢＩ。ＢＩ能抑制多种植物病原菌的生长,对热稳定,对蛋白酶部分敏感。经ＳＤＳ－ＰＡＧＥ和等电聚焦电泳测定其分子量约１４．５ｋＤ,等电点为５．５８。氨基酸组成分析表明,该蛋白宫含谷氨酸、酪氨酸和脯氨酸;并测定了Ｎ末端氨基酸的部分序列。     

γ-射线及大肠杆菌诱导蓖麻蚕产生抗菌物质的研究

1.用γ-射线辐照和用大肠杆菌处理蓖麻蚕五龄幼虫和蚕蛹均能诱导血淋巴产生抗菌物质,两种诱导源诱导所得活性物质的抗菌活性相似.2.研究了五龄幼虫期和蛹期诱导产生抗菌物质的动力学,发现五龄幼虫在饷食后第2—4天诱导活力最高,产生抗菌物质的持续时间亦较长;蛹期则从化蛹当天至第4天之间诱导活力较高,并可持续15天左右,高峰期一般在诱导后2天至4天之间.3.对诱导后的蓖麻蚕血淋巴进行了电泳测活和葡聚糖凝胶初步分离,发现不论幼虫期或蛹期至少可得三个活性组分,其中既有类似于P₅的大分子抗菌物质,也有类似于P_9A和P_9B的抗菌多肽;并首次发现一种分子量约70000—75000道尔顿的新抗菌蛋白.     

可溶性BVP功能树脂组成对抗菌活性的影响

系统地研究了可溶性BVP树脂对Escherichiacoli的抗菌作用,探讨了树脂的吡啶盐含量、平衡离子类型、第二单体及R1基团结构、分子量及聚合方法等对其抗菌活性的影响。     

蝇源抗菌肽的研究进展

抗菌肽是阳离子型活性肽,是昆虫防御体系的重要组成部分,具有分子量小、热稳定性好、无免疫原性、广谱抗菌等特点。就蝇源抗菌肽种类、抗菌机理及其研究展望和存在问题进行了综述。     

某些抗菌肽的研究进展

抗菌肽是各种生物防御系统的一个组成部分,是由于微生物等因素的侵染而产生的免疫应答反应产物,具有分子量低,热稳定,强碱性和广谱抗菌等特点,抗菌肽的正电荷与细菌细胞的磷脂头负电荷之间的相互作用是重要,肽分子氮端的两性螺旋是裂解细菌的主要部分,碳末端酰胺化与抗菌肽的广谱抗菌有关,抗菌肽具有独特的抗菌机理,能在细菌质膜上形成离子通道,破坏膜势,引起胞内物质泄漏,从而杀灭细菌。     

Bacillus subtilis fmbJ脂肽类抗菌物质的分离和鉴定

对BacillussubtilisfmbJ脂肽类抗菌物质的分离和鉴定进行了系统研究。通过HPLC层析确定BacillussubtilisfmbJ抗菌物质由多种组分构成,其中含有保留时间与surfactin相似的成分。通过TLC层析和原位酸解确定BacillussubtilisfmbJ抗菌物质含有两个具有闭合肽键类的物质,其中之一为迁移率Rf与标样surfactin非常相近的组分。通过ESI-MS分析检测到BacillussubtilisfmbJ抗菌物质含有分子量与fengicin相同的m/z1449.9、m/z1463.8、m/z1477.8、m/z1491.9和m/z1505.9五种同系物,和分子量与surfactin相同的m/z1008.8、m/z1022.8和m/z1036.8三种同系物。     

可溶性BVP功能树脂组成对抗菌活性的影响*

系统地研究了可溶性BVP树脂对Escherichiacoli的抗菌作用,探讨了树脂的吡啶盐含量、平衡离子类型、第二单体及R1基团结构、分子量及聚合方法等对其抗菌活性的影响。     

Properties of prolamin in mature and developing rice grain

A procedure was developed for preparing lipid- and phenol-free prolamin directly from IR480-5-9 milled rice (Oryza sativa L.).The preparation consisted mainly of one protein band on analytical and SDS-polyacrylamide disc gel electrophoresis with subunit MW of 17000 and a minor fraction with subunit MW 23000. The prolamin eluted as a single peak on SDS-Sephadex G-75 gel filtration and on DEAE-cellulose column chromatography. Prolamin was poor in lysine, histidine, cystine, and methionine but rich in glutamic acid, tyrosine and proline. In dehulled developing grain of two different rices, changes in the aminogram of the prolamin fraction coincided with the start of endosperm protein body synthesis and the appearance from 7 days after flowering of a second prolamin subunit with MW 23 000.     

Purification of modulator-deficient myosin light-chain kinase by modulator protein-Sepharose affinity chromatography.

Modulator-deficient myosin light-chain kinase from rabbit skeletal muscle was purified by modulator protein-Sepharose 4B affinity chromatography. The purified protein showed a single band (MW 80,000) on polyacrylamide gel electrophoresis in sodium dodecyl sulfate, and it exists as a monomer in the native state as determined by gel filtration. The modulator-deficient myosin light-chain kinase (MW 80,000), modulator protein (MW 16,500) and Ca2+ were essential for the kinase activity. The half-maximal activity of the kinase in the presence of excess modulator protein with 10 mM MgCl2 was at pCa 5.1, where full activity of actomyosin-ATPase is observed in the presence of the troponin--tropomyosin system. Assuming a rapid equilibrium between myosin light-chain kinase and two substrates, ATP and g2 light-chain, Km values for ATP and g2 light chain were evaluated as 0.28 mM and 0.024 mM, respectively. Vm/e was 5.7 s-1.     

Isolation of Secretory IgA from a Lung Surfactant Fraction

Although dipalmitoyl lecithin, is the essential component of the pulmonary surfactant system that is invoked for alveolar stability, there is no explanation as yet for the origin and role of certain proteins that are found with the phospholipid in pulmonary washings. Aqueous lavages obtained from rabbit lung contain three major proteins, two of which are serum proteins (albumin 60%, γ-globulin 10%), and the third, protein “T” (20%), is described here as pulmonary secretory immunoglobulin A (sIgA). The protein is first recovered quantitatively in the surface activelipid -protein fraction from filtration of pulmonary lavage on Sephadex G-200. The protein is then isolated from the lipid either by filtration on SDS-Sephadex G-200 or by ethanol-ether precipitation. After reductive cleavage with either mercaptoethanol or dithiothreitol and alkylation with iodoacetamide, three protein peaks are obtained from SDS-sephadex G-200 separation. The products of reductive cleavage are analogous to the secretory component (MW～60,000), H-chain (MW～50,000), L-chain (MW～25,000), and J-piece (MW～28,000) of secretory IgA frm colostrum. In inmunodiffusion the lung protein and colostrum sIgA show striking identity lines, as do antibodies to rabbit colostrum and to the lung protein. Amino acid and carbohydrate analyses reveal some differences between the two secretory immunoglobulins. Although this protein has been found together with the phospholipid surfactant of the lung in vitro, the present structural study concludes that the protein is SIgA. Although concurrent immunof luorescence studies showed that this protein is in the alveolar lining layer, we cannot as yet conclude that it belongs to the surfactant system of the lung.     

The latency of spinach chloroplast phenolase

The latent phenolase in spinach chloroplast membranes could be activated by treatment with various detergents. Examination by thin-layer gel filtration showed the presence of two active proteins (one with lower MW called protein A and the other, protein B). The protein B was converted to A by dilution or on standing, and the latter conversely to the former by concentration. On freezing, an extract of the acetone powder of the chloroplasts, phenolase activity was strikingly reduced, and this is ascribed to an association of the protein A and a low MW (diffusible) substance giving rise to an inactive enzyme-inhibitor complex. The activity declined from autumn to winter, and it appears that the second type of latency due to the formation of the above complex is also involved.     

Evidence for selenocysteine in ovine tissue organelles

Subcellular fractions were prepared by differential centrifugation from heart and liver of a lamb labeled with 75Se-selenite. Crude fractions of nuclei, mitochondria, and microsomes from both tissues were solubilized with sodium dodecyl sulfate and chromatographed on columns of sephacryl S-200. A low molecular weight (MW) 75Se labeled cardiac cytosol protein (approximately 10,000 daltons) was partially purified by gel filtration chromatography. The major 75Se peaks from the sephacryl columns and the low MW cardiac protein were hydrolyzed in HCl under an inert atmosphere. When chromatographed on an amino acid analysis column, 75Se from each hydrolysate chromatographed in the identical position of 2,7-diamino-4-thia-5-selenaoctanedioic acid, the mixed oxidized dimer of cysteine and selenocysteine. The low MW cardiac protein was reacted with chloroacetate after reduction with borohydride. 75Se from a hydrolysate of this derivatized protein eluted in the same position as Se-carboxymethylselenocysteine on the amino acid analysis column. Thus, selenocysteine appears to be the predominant form of selenium in ovine heart and liver.     

Hydrophobic chromatographic purification of ethylene-enhanced chlorophyllase from Citrus unshiu fruits

Ethylene-enhanced chlorophyllase from Citrus unshiu fruits was purified to a homogeneous state after solubilization with sodium cholate, using acetone precipitation and hydrophobic chromatography. The enzyme adhered to phenyl Sepharose CL-4B in 3M KCl and was eluted with a linear gradient of Triton X-100 (0–0.5%). Its MW (SDS-PAGE) was 27 000. The enzyme behaved as a protein of MW 110 000 on Sephacryl S-200 gel filtration. The enzyme showed a specific activity of 0.069 μamol chlorophyllide a produced/min/ mg protein. This purification procedure is a rapid method for obtaining pure chlorophyllase.     

牛脑中神经特异性S-100蛋白的纯化及鉴定

牛脑充分匀浆后经三次硫酸铵分级沉淀,再通过一次DEAE-Sepharose CL-6B层析柱,线性梯度洗脱后共收集4个峰洗脱液。PAGE分析(7.5％凝胶)显示第3峰为单一区带;免疫双扩散证实该洗脱液中蛋白为S-100蛋白。SDS-PAG E分析显示S-100蛋白分子量约为10kD;非还原条件下,凝胶过滤(Sephadex G-75)显示S-100蛋白位于MW为20kD区域。认为该纯化方法简便、快速,可获得较高纯度的S-100蛋白,活性高达1∶128以上,完全能满足进一步研究之用。     

Properties and Partial Purification of Choline Acetyltransferase from the Nematode Caenorhabditis elegans

We have stabilized and studied choline acetyltransferase from the nematode Caenorhabditis elegans. The enzyme is soluble, and two discrete forms were resolved by gel filtration. The larger of these two forms (MW approximately 154,000) was somewhat unstable and in the presence of 0.5 M NaI was converted to a form indistinguishable from the "native" small form (MW approximately 71,000). We have purified the small form of the enzyme greater than 3,300-fold by a combination of gel filtration, ion-exchange chromatography, and nucleotide affinity chromatography. The purified preparation has a measured specific activity of 3.74 mumol/min/mg protein, and is free of acetylcholinesterase and acetyl-CoA hydrolase activities. The Vmax of the purified enzyme is stimulated by NaCl, with half-maximal stimulation at 80 mM NaCl. The Km for each substrate is also affected by salt, but in different manners from each other and the Vmax; the kinetic parameter Vmax/Km thus changes significantly as a function of the salt concentration.     

杏鲍菇抗烟草花叶病毒蛋白的筛选

采用离子交换层析和凝胶层析方法,从杏鲍菇干样中分离得到多个蛋白组分,经枯斑寄主检测,发现多个蛋白组分都有抗烟草花叶病毒(TMV)的活性,对TMV的抑制率均在70%以上,高者可达99%。其中xb68Ab已得到了纯化,分子量约为23.7kD,在心叶烟和苋色藜上它对TMV侵染的抑制率分别达到99.43%和98.9%。     

Chemical and Immunological Characterization of a Low Molecular Weight Outer Membrane Protein of Salmonella typhi

A new immunogenic outer membrane protein, Omp-28 (MW 28,000 and pI 4.6), was isolated from smooth Salmonella typhi cells by the use of an extracting medium containing 6 m urea, 1% deoxycholate and 5 mM EDTA. The purification of Omp-28 was performed by gel filtration and fast ion exchange chromatography. This protein showed to be the prevalent component isolated by the latter methodology. Omp-28 is formed by three identical subunits (MW 9,000), not linked by disulfide bonds. The partial N-terminal amino acid sequence of Omp-28 presented great homology with part of the sequence of an Escherichia coli protein found in a precursor whose sequence was predicted by c-DNA. ELISA and Western blotting identified Omp-28 as the major antigenic protein present in the outer membrane protein fraction, isolated by gel filtration. Antibodies against Omp-28 were detected by ELISA in 43% of 28 sera from typhoid fever convalescent patients. The antisera from mice immunized with Omp-28 and the highest positive typhoid fever convalescent serum gave a positive bactericidal test, killing 50% of Salmonella typhi cells in serum dilutions of 1/80 and 1/320, respectively. These results indicate the immunogenic importance of Omp-28 isolated from Salmonella typhi outer membrane and strongly suggest it should be used in further studies of animal protection against the disease caused by this pathogenic bacteria.