Enzymatic Detoxification of HC-toxin, the Host-Selective Cyclic Peptide from Cochliobolus carbonum

Resistance to the fungal plant pathogen Cochliobolus carbonum race 1 and to its host-selective toxin, HC-toxin, is determined by Hm, a single dominant gene in the host plant maize, (Zea mays L). Radiolabeled HC-toxin of specific activity 70 milliCuries per millimole, prepared by feeding tritiated d,l-alanine to the fungus, was used to study its fate in maize leaf tissues. HC-toxin was converted by resistant leaf segments to a single compound, identified by mass spectrometry and nuclear magnetic resonance as the 8-hydroxy derivative of HC-toxin formed by reduction of the 8-keto group of 2-amino-9, 10-epoxy-8-oxo-decanoic acid, one of the amino acids in HC-toxin. Reduction of HC-toxin occurred in cell-free preparations from etiolated (Hm/hm) maize shoots, and the activity was sensitive to heat and proteolytic digestion, dependent on NADPH, and inhibited by p-hydroxymercuribenzoate and disulfiram. The enzyme (from the Hm/hm genotype) was partially purified by ammonium sulfate precipitation and diethylaminoethyl-ion exchange chromatography. By gel filtration chromatography, the enzyme had a molecular weight of 42,000. NADH was approximately 30% as effective as NADPH as a hydride donor, and flavin-containing cofactors had no effect on activity. When HC-toxin was introduced to maize leaf segments through the transpiration stream, leaf segments from both resistant and susceptible maize inactivated toxin equally well over a time-course of 9 hours. Although these data suggest no relationship between toxin metabolism and host selectivity, we discuss findings in apparent conflict with the current data and describe why the relationship between enzymatic reduction of HC-toxin and Hm remains unresolved.     

Molecular Genetic Features of Biological Species of the Genus Saccharomyces

Microbiology - Molecular genetic study of Saccharomyces yeasts of different species was carried out using molecular karyotyping and comparative analysis of a number of nuclear and mitochondrial...     

Isolation and Biological Activities of Four Selective Toxins from Helminthosporium carbonum

A new and simpler purification procedure was developed for host selective toxins from Helminthosporium carbonum race 1. Four analogs or forms of toxin with the same selectivity as the fungus were isolated from culture fluids; two forms (HC toxins III and IV) have not been reported by other workers. Crystals of the major form of toxin (HC toxin I) were recovered in high yields (>80 milligrams per liter of culture fluid) without the use of high performance or preparative thin layer liquid chromatography. ED₅₀ values, based on inhibition of root growth of susceptible seedlings, for HC toxins I, II, III, and IV were 0.2, 0.4, 2.0, and 20 micrograms per milliliter, respectively. The specific activity of crystalline HC toxin I matched the most active preparation reported previously; the preparation of HC toxin II was more active than that reported previously. Resistant seedlings tolerated 100-fold higher concentrations of each form of toxin than did susceptible seedlings. Hydrolysis of the epoxide group of HC toxin I to a diol destroyed toxicity to susceptible and resistant seedlings. The data suggest that the same mechanisms are affected in resistant and susceptible plants.     

嗜热脱铁去硫弧菌Pif1解旋酶生物学活性的分子特征分析

已知Pif1解旋酶在维持基因组稳定性方面发挥重要作用,且不同生物Pif1解旋酶具有不同的生物学活性;然而迄今为止,嗜热细菌Pif1解旋酶的生物学活性分子特征的研究尚未见报道。本文运用生物化学与生物物理学前沿技术,系统地研究了嗜热脱铁去硫弧菌Pif1解旋酶（Defe.Pif1）结合活性与解旋活性的分子特征。通过原核表达纯化系统,本研究获得纯度95%以上、无标签的Defe.Pif1蛋白。利用荧光偏振技术研究Defe.Pif1结合反应的底物特异性,揭示出Defe.Pif1优先结合ssDNA与G4 DNA,并对含3′-尾链的部分双链底物有较强亲和力,其结合反应底物特异性为：ssDNA > G4 DNA > 3′-ssDNA-dsDNA≈Y-structure > Other substrates。通过快速停留检测技术研究Defe.Pif1的解旋活性,明确其最适解旋温度为50℃,最佳反应溶液为10 mmol/L NaCl、3 mmol/L DTT、3 mmol/L MgCl2及1 mmol/L ATP;进一步的解旋动力学特征分析结果显示,Defe.Pif1可以高效解旋含G4结构的DNA底物,其解旋5′-G4 dsDNA底物时的解旋幅度超过90%,解旋速率也与其解旋5′-ss-dsDNA底物的速率相近,提示Defe.Pif1解旋G4 DNA更接近Bs.Pif1的单体反应模式。此外,本研究还发现Defe.Pif1解旋不同类型复制叉/复制泡底物时拥有独特的解旋倾向性：与解旋其它复制中间体DNA的低效性不同,Defe.Pif1解旋12nt bubble底物的速率与幅度均较高,暗示12nt bubble结构很可能是该解旋酶复制中间体的天然底物。上述结果证明,Defe.Pif1不仅具有Pif1解旋酶家族成员共同的结合与解旋G4 DNA等活性特征;而且作为嗜热细菌的解旋酶,它还具有独特的反应条件与解旋底物特异性。本研究为研究Pif1解旋酶家族其它成员的分子特征与生物功能提供了潜在的研究策略,为阐明此类Pif1解旋酶的分子作用机制奠定实验基础。     

A novel alcohol oxidase/RNA-binding protein with affinity for mycovirus double-stranded RNA from the filamentous fungus Helminthosporium (Cochliobolus) victoriae: molecular and functional characterization

We have cloned and sequenced a novel alcohol oxidase (Hv-p68) from the filamentous fungus Helminthosporium (Cochliobolus) victoriae that copurifies with mycoviral double-stranded RNAs. Sequence analysis revealed that Hv-p68 belongs to the large family of FAD-dependent glucose methanol choline oxidoreductases and that it shares significant sequence identity (>67%) with the alcohol oxidases of the methylotrophic yeasts. Unlike the intronless alcohol oxidases from methylotrophic yeasts, a genomic fragment of the Hv-p68 gene was found to contain four introns. Hv-p68, purified from fungal extracts, showed only limited methanol oxidizing activity, and its expression was not induced in cultures supplemented with methanol as the sole carbon source. Northern hybridization analysis indicated that overexpression of Hv-p68 is associated with virus infection, because significantly higher Hv-p68 mRNA levels (10- to 20-fold) were detected in virus-infected isolates compared with virus-free ones. We confirmed by Northwestern blot analysis that Hv-p68 exhibits RNA binding activity and demonstrated that the RNA-binding domain is localized within the N-terminal region that contains a typical ADP-binding beta-alpha-beta fold motif. The Hv-p68 gene, or closely similar genes, was present in all species of the genus Cochliobolus but absent in the filamentous fungus, Penicillium chrysogenum, as well as in two nonmethylotrophic yeasts examined. This study represents the first reported case that a member of the FAD-dependent glucose methanol choline oxidoreductase family, Hv-p68, may function as an RNA-binding protein.     

Selective Toxins and Analogs Produced by Helminthosporium sacchari: Production, Characterization, and Biological Activity

Helminthosporium sacchari toxin and several lower molecular weight, nontoxic analogs were isolated from culture filtrates. Three isomers of the toxin (A, B, and C), each with four galactose units, were separated by high performance liquid chromatography. Isomer C had the highest and isomer A had the lowest toxicity to H. sacchari-susceptible sugarcane; resistant clones were not affected. Each toxin isomer was partially digested with a β-galactofuranosidase and the resulting analogs (seven from each toxin isomer) were separated by reverse phase high performance liquid chromatography and identified. Each isomer of the analogs with 3 galactose units per mole also was partially digested and the arrangement of galactose units was determined. The compound with one galactose attached to position 2 of the bicyclic sesquiterpene and with 2 galactose units attached to position 13 (analog A_1,2) was highly toxic to some but not to all clones of H. sacchari-susceptible sugarcane. Toxin analogs protected sensitive tissue against active toxin; protective effects of the analogs differed, but at least a 10-fold excess of analog was required. Analog C_2,1 was more effective at preventing toxin C-induced electrolyte losses than was any other analog. Each of the 3-galactose analog isomers protected better than did any of the 2-galactose compounds. The 1,1 analogs did not protect as well as did the 2,0 or 0,2 analogs. Thus, the sesquiterpene isomer, the number of galactose units, and the galactose arrangement pattern determine the effectiveness of the compound in induction of electrolyte loss and in prevention of toxininduced loss from sugarcane tissues.     

Effect of the Molecular Chain Length on Biological Activity of Juvenile Hormone Analogs

Twenty six juvenile hormone analogs with various molecular chain length were prepared and bioassayed using allatectomized 4th instar larvae of Bombyx mori L. Among methyl or ethyl esters, the chain length of 17 atoms is the optimal for the high juvenile hormone activity on the silkworm.     

Biological Activity of Polar Lipids from Bifidobacteria

Fractions of polar lipids have been isolated from bifidobacteria, and the immunoreactivity and serological specificity of glycolipids and phospholipids have been studied. Enzyme immunoassay (dot-EIA) of polar lipids demonstrates that the fractions of glycolipids and phospholipids of bifidobacteria are highly immunoreactive. Pronounced reactions of major glycolipids and phospholipids with a homologous polyvalent antiserum against B. adolescentis 94-BIM have been observed at antigen concentrations of approximately 100 ng. The antiserum contained high titers of specific antibodies against glycolipids and phospholipids of bifidobacteria, as demonstrated by heterogeneous solid-phase enzyme immunoassay (ELISA). Experimental data confirming the presence of subpopulations of specific antibodies (antiglycolipid and antiphospholipid) in the blood sera of immunized animals lead to the conclusion that the major glycolipids and phospholipids of bifidobacteria are specific markers appropriate for serological diagnostics.     

截短型细胞毒素Gelonin的分子构象和生物活性

为了探索免疫络合物中具杀伤靶细胞的毒素,gelonin的结构与功能的关系,根据化学合成的gelonin基因序列和3维分子构象设计了N端区Gly,Leu,Asp和/或C端区Asp,Lys,Asp,Pro,Lys缺失的gelonin. 以重组质粒pE gel为模板,在相应引物存在下,用PCR法获得5′端区和/或3′端区碱基序列缺失的gelonin基因片段. 经克隆、表达和纯化得到3种截短型gelonin（G-N3、G-C5、G-N3C5）. CD谱和荧光谱表明,完整型gelonin（G-O）与截短型gelonin的分子构象有明显的差异.它们的构象变化与类DNase活性和抑制肿瘤细胞生长的能力均为G-O≥ G-N3＞G C5＞G-N3C5. 结果再一次证明了具有α+β型结构蛋白,gelonin的构象与生物活性的一致性.     

Correlative Analysis of Cochliobolus sativus Pathogenicity and in vitro Xylanase Activity

Spot blotch (SB) caused by Cochliobolus sativus has been the major yield‐reducing factor for barley production during the last decade. In this study, the correlation between aggressiveness and in vitro xylanase production of 29 isolates of C. sativus was investigated. Isolate aggressiveness was evaluated in term of lesion form in barley leaves. Additionally, the isolates were compared for their ability to produce in vitro significant levels of xylanase activities when grown in a liquid medium. Aggressive isolates released more xylanase of weakly aggressive isolates. Correlation tests analysis revealed a significant relationship (r = 0.84, r = 0.50; P < 0.01) between the xylanase (per unit fungal mass) and aggressiveness on the two barley cultivars Arabi Abiad and Bowman, respectively. Correlation between the production of this enzyme and the origin of the isolates was not found. The results indicate that the production of xylanase influences the aggressiveness of the isolates of C. sativus towards barley seedlings.     

Factors Affecting the Activity of Cellulases Isolated from the Rumen Digesta of Sheep

Sodium phosphate buffer was used to extract cellulases from the plant solids fraction of rumen contents. The mixed cellulase preparation had maximal activity at pH 6.9 and 49°C. The V_max and the apparent K_m for wheaten hay cellulose were 19.8 glucose units/min and 6.35 mg/ml, respectively, and for microcrystalline cellulose (Sigmacell) at the same enzyme concentration, they were 33 glucose units/min and 27.5 mg/ml, respectively. For these assays a glucose unit was defined as nanomoles of glucose plus twice the nanomoles of cellobiose. Consideration of thermodynamic and kinetic data suggested that the hydrolysis of a relatively labile arabino-xylan comprising 3% of the wheaten hay cellulose was dependent on prior removal of the protecting β-1,4-glucose chains at the outer surface of the cellulose preparation. Sequential removal of structural polysaccharides from the plant cell wall rendered the latter more susceptible to cellulase activity. Cellulase activity was stimulated by increasing the concentration of phosphate from 5 to 50 mM. The stimulation was magnified in the presence of cell-free rumen fluid. Cellulase activity was not stimulated by calcium, magnesium, iron, zinc, manganese, copper, or cobalt ions and was unaffected by the chelators ethylenediaminetetraacetic acid and ethyleneglycol-bis (β-aminoethyl ether)-N,N′-tetraacetic acid. O-phenanthroline inhibited activity by 30 to 50%, but this may have been due to nonchelate properties. Anaerobic conditions or thiol protective agents were not essential for either the activity or stability of the cellulases during assay. An ultrafiltrable inhibitor of cellulase activity was detected in cell-free rumen fluid.     

The Use of Chitosan Salicylate to Increase the Biological Efficiency of Vitaplan against Cochliobolus sativus

Applied Biochemistry and Microbiology - The possibility of increasing the biological efficiency of the Vitaplan biological product via the inclusion of chitosan salicylate as an inducer of plant...     

Factors Affecting the Activity of Phenolic Disinfectants

Low challenge phenol coefficient and high challenge use-dilution tests were made on a neutral cocoanut oil soap emulsion of o-phenylphenol and aqueous solutions of sodium o-phenylphenate prepared in the laboratory from the phenol using a stoichiometric amount of NaOH as well as with increasing amounts of excess NaOH. The phenol had considerably greater activity in both test methods when emulsified with the neutral soap than when converted to the phenate and dissolved in water. Use dilution test results against Salmonella choleraesuis with both the phenol and the phenate were within the range which would have been predicted from the Salmonella typhosa coefficient results employing the conventional conversion multiple of 20 to determine the maximal number of parts of water to which one part of germicide could be added. With the emulsified phenol this was also true where Staphylococcus aureus was employed in both procedures. With the aqueous solution of the phenate the maximal safe use-dilution by the phenol coefficient found for S. aureus and the same conventional conversion procedure was roughly five times higher than the maximal safe use-dilution found by the use-dilution method. Results with aqueous solutions of the phenate to which increasing amounts of excess NaOH were added showed no significant differences in the phenol coefficient method with either S. typhosa or S. aureus. In the use-dilution method, significant decreases in activity were found as the excess NaOH was increased to 4% with both S. choleraesuis and S. aureus. Although the pH values of aqueous solutions of the phenate were raised as the amount of free NaOH was increased, the decreases in pH observed as the dilution with water was increased were such that only small differences existed at the high critical killing dilutions found in the low challenge phenol coefficient method, whereas rather large differences existed at the lower critical killing dilutions in the high challenge use-dilution method.     

神经生长抑制因子相互作用蛋白的分子克隆、鉴定及其生物学特性

为了探讨神经生长抑制因子(Neuronal growth inhibitory factor,GIF)与Alzheimer’s病(Alzheimer’s disease,AD)的关系,将GIF的cDNA全基因克隆到载体pHyblex中,运用酵母双杂交系统从Alzheimer’s病人脑cDNA文库中筛选出与GIF相互作用蛋白的cDNA克隆。免疫共沉淀和蛋白质印迹实验进一步验证了该蛋白在体内与GIF相互作用的特异性。克隆并鉴定了其中1个与GIF特异性结合的蛋白,与人细胞核dUTP焦磷酸酶(DUT)同源。进一步构建了重组表达质粒pGEX-4T-1／DUT,转化大肠杆菌BL21,经谷胱甘肽-Sepharose 4B亲和层析、凝血酶酶切和Sephacryl S100纯化,得到纯度95％以上的dUTPase蛋白。体外生物学活性检测表明,表达的dUTPase蛋白可以与GIF共同作用嗜铬细胞瘤株(pheochromocytoma)PC12,对细胞的生长产生抑制作用。     

Dynamic Diversification from a Putative Common Ancestor of Scorpion Toxins Affecting Sodium, Potassium, and Chloride Channels

Scorpions have survived successfully over millions of years without detectable changes in their morphology. Instead, they have developed an efficient alomonal machinery and a stinging device supporting their needs for prey and defense. They produce a large variety of polypeptidic toxins that bind and modulate ion channel conductance in excitable tissues. The binding site, mode of action, and chemical properties of many toxins have been studied extensively, but little is known about their genomic organization and diversity. Genes representing each of the major classes of Buthidae scorpion toxins, namely, ``long' toxins, affecting sodium channels (alpha, depressant, and excitatory), and ``short' toxins, affecting potassium and chloride channels, were isolated from a single scorpion segment and analyzed. Each toxin type was found to be encoded by a gene family. Regardless of toxin length, 3-D structure, and site of action, all genes contain A+T-rich introns that split, at a conserved location, an amino acid codon of the signal sequence. The introns vary in length and sequence but display identical boundaries, agree with the GT/AG splice junctions, and contain T-runs downstream of a putative branch point, 5′-TAAT-3′. Despite little sequence similarity among all toxin classes, the conserved gene organization, intron features, and common cysteine-stabilized α-helical (CSH) core connecting an α-helix to a three-stranded β-sheet suggest, that they all evolved from an ancestral common progenitor. Furthermore, the vast diversity found among genomic copies, cDNAs, and their protein products for each toxin suggests an extensive evolutionary process of the scorpion ``pharmaceutical factory,' whose success is due, most likely, to the inherent permissiveness of the toxin exterior to structural alterations. Received: 16 March 1998 / Accepted: 30 July 1998     

Factors Affecting the Cellulolytic Activity of Rumen Contents

The cellulolytic activity of rumen contents was assayed by measuring losses in weight and tensile strength of cotton yarn incubated in rumen contents in the presence of dietary additives (barley, tallow) and at different pH values. The addition of barley depressed cellulolysis and the titer of filter paper-degrading bacteria only if the pH was allowed to fall. Lowering the pH from 7.0 to 6.0 by addition of HCl almost completely inhibited attack of cotton and greatly reduced the titer of filter paper-degrading bacteria. The layering of tallow on cotton inhibited attack of cotton but did not decrease the titer of filter paper-degrading bacteria. The results are discussed with special reference to the importance of the study of cellulosic substrates, which require a known enzyme or mixture of enzymes for attack.     

Biological Activity of Purpurogallin

Purpurogallin showed antibacterial activity toward gram-positive bacteria. Strong activity against methicillin-resistant Staphylococcus aureus [minimal inhibitory concentration (MIC) against methicillin of 1600 μg/ml] was found, with MIC of 11.0/μg/ml. Purpurogallin inhibited the growth of all tested plants and decreased the chlorophyll content in the cotyledons of Brassica campestris subsp. rapa. It showed potent inhibitory activity against prolyl endopeptidase (the 50% inhibitory concentration was 1.6 × 10^?5m), unlike its analogues, hinokitiol and tropolone.