芹菜夜蛾核型多角体病毒D克隆株某些理化性质的研究

DNA of Syngrapha falcifera nuclear polyhedrosis virus D-clone(Sfa-D clone) was extracted and digested by three kinds of restriction endonuclease,We calculated its molecular weight and measure its melting temperature,G C%, virus particle and polyhedrin were purified.The structural polypeptides and polyhedrin are analysed by SDS-PAGE.     

两株粘虫核型多角体病毒理化性质的比较研究

电镜观察粘虫(Leucania separala)核型多角体病毒的不同株系内蒙株(简称N株)和阜阳株(简称F株)的多角体、病毒粒子及核衣壳在形态大小方面都没有很大差别,DNA分子大小也相近。但在SDS-PAGE多肽图谱及DNA酶切图谱上则表现出一定的差异。经SDS-PAGE所得病毒粒子多肽图谱N株有17条多肽,F株有19条多肽。两株病毒DNA经BamHI酶切N株获得7条带,F株则有8条带,说明DNA酶切位点不尽相同。据此,生化分析能更快速、准确地进行株系分类。     

棉铃虫核型多角体病毒朝鲜分离株的初步研究

为了充分利用棉铃虫核型多角体病毒(Helicoverpa armigera,HaSNPV)资源,为开展害虫生物防治提供依据,对首次在朝鲜分离到的棉铃虫核型多角体病毒进行了研究.本文从形态结构,结构多肽.核酸限制性内切酶图谱等方面进行了研究.多角体直径0.36-1.3 μm,平均1.02μm,病毒粒子大小为326 nm×69nm.经SDS-PAGE分析,棉铃虫核型多角体朝鲜株多角体蛋白为一条带.多角体蛋白分子量为28.7kDa.棉铃虫核型多角体朝鲜株基因组经BamH I,EcoR I,HindⅢ和Pst I消化后,得到的内切酶图谱表现,与已报道的几个分离株比较类似.分子大小均为130.18kb.     

灰茶尺蛾核型多角体病毒某些生化特性的研究

灰茶尺蛾核型多角体病毒某些生化特性的研究李彦章,石正丽,陈棣华（中国科学院武汉病毒研究所,武汉４３００７１）关键词灰茶尺蛾,核型多角体病毒,结构多肽,限制性内切酶图谱灰茶尺蛾核型多角体病毒（Ｅｃｔｒｏｐｉｓｇｒｉｓｅｓｃｅｎｓｎｕｃｌｅａｒｐｏｌｙｈ...     

扁刺蛾核型多角体病毒的形态结构与某些生化特性的测定

扁刺蛾核型多角体病毒是一种单粒包埋型的杆状病毒,在扫描电镜下呈不规则多面体。病毒多角体大小不一致,平均直径为0.59μ。病毒粒子为340×85nm. 经SDS—PAGE分析,病毒的多角体蛋白主带分子量为29500道尔顿;病毒粒子的结构蛋白具有25条多肽,分子量为17.8～69.5×10~4道尔顿。病毒多角体蛋白氨基酸组成中富含Asp和Glu,而His、Cys、Met的含量却很低。病毒DNA的分子量为67.89×10~6道尔顿。     

乌桕金带蛾核型多角体病毒的理化性质和内切酶分析

1985年我们从自然罹死的乌桕金带蛾(Eupterote sapivora yang)幼虫分离到一株核型多角体病毒,经电镜观察认为是杆状病毒属(Baculovirus)中的一种病毒(简称EsNPV)。研究昆虫病毒的分子遗传学及基因重组和表达,制备安全有效的昆虫病毒杀虫剂等,首先都要纯化病毒,对其理化性质需要有较全面的了解。为此,本文对该病毒的理化性质和限制性     

蜀柏毒蛾核型多角体病毒结构多肽及基因组酶切分析

对蜀伯毒蛾核型多角体病毒（Ｐａｒｏｃｎｅｒｉａ ｏｒｉｅｎｔａ Ｎｕｃｌｅａｒ ｐｏｌｙｈｅｄｒｏｖｉｒｕｓ,简称ＰａｏｒＮＰＶ）形态结构、结构多肽、限制内切酶图谱等特性进行了研究。采用不连续系统垂直板ＳＤＳ－ＰＡＧＥ分析了ＰａｏｒＮＰＶ的多角体蛋白、病毒粒子结构多肽。应用５种限制性内切酶对ＰａｏｒＮＰＶ基因组ＤＮＡ进行了酶切分析。结果表明：经热处理的多角体蛋白仅有一条带,分子量为３１．５ｋＤ,不     

棉铃虫（Heliothisspp）核型多角体病毒四个分离株的比较研究

本文从形态结构、生物活性、结构多肽、核酸限制性内切酶图谱和核酸同源性等方面对棉铃虫核型多角体病毒四个分离株（两个ＳＮＰＶ分离株：ＨａＳ、ＨｚＳ,和两个ＭＮＰＶ分离株：ＨａＭ１、ＨａＭ２）进行了比较研究。它们对中国棉铃虫二龄末三龄初幼虫的ＬＤ５０佰依次为３６１、３８７、２６３３、３５６０ＰＩＢｓ／克饲料,当感染剂过为５×ｌ０３ＰＩＢｓ／克饲料时,其ＬＴ５０值依次为４．６、４．９、６．４和６．６天。两个ＳＮＰＶ分离株的生物活性显著高于两个ＭＮＰＶ分离株。经ＳＤＳ－ＰＡＧＥ分析,四个分离株多角体蛋白均为一条带,两个ＭＮＰＶ分离株结构多肽均具有相同的迁移率,两个ＳＮＰＶ分离株的结构多肽图谱也颇相似,但ＳＮＰＶ与ＭＮＰＶ分离株之间带型相差较大。各分离株基出组经ＢａｍＨＩ、ＥｃｏＲＩ、ＨｉｎｄⅢ和ＸｂａＩ消化后,得到的内切酶图谱表现为两个ＮＭＰＶ分离株一致,两个ＳＮＰＶ分离株也很相似,而ＳＮＰＶ与ＭＮＰＶ分离株之间相差很大。严格条件杂交结果表明：两个ＳＮＰＶ分离株的基因组有较高的同源性,而ＳＮＰＶ与ＭＮＰＶ基因组之间的同源性极低。     

三种夜蛾科昆虫核型多角体病毒DNA相关性的研究

核型多角体病毒属杆状病毒科,主要感染鳞翅目、双翅目和膜翅目的昆虫,具有90～160kb长的双链,超螺旋DNA基因组。现已发现约500种核型多角体病毒,这些病毒之间有什么关系？它们的亲缘关系如何？我们以甘兰夜蛾核型多角体病毒（简称MbNPV）、甜菜夜蛾核型多角体病毒（简称SeNPV）和斜纹夜蛾核型多角体病毒（简称SINPV）为材料,用限制性内切酪和分子杂交技术对它们的基因组DNA进行比较研究,并对其中一种病毒MbMV多角体蛋白基因进行了定位,现将结果报道如下;材料和方法1材料甜菜夜蛾和斜纹夜蛾健康幼虫,病毒麦种MbNPV、SeN…     

蜀柏毒蛾核型多角体病毒结构多肽及基因组酶切分析

对蜀柏毒蛾核型多角体病毒(Parocneria orienta Nuclear polyhedrovirus,简称PaorNPV)形态结构、结构多肽、限制性内切酶图谱等特性进行了研究.采用不连续系统垂直板SDS-PAGE分析了PaorNPV的多角体蛋白、病毒粒子结构多肽.应用5种限制性内切酶对PaorNPV基因组DNA进行了酶切分析.结果表明:经热处理的多角体蛋白仅有一条带,分子量为31.5 kD,不经热处理的多角体蛋白有三条带,分子量分别为31.5 kD、29.1 kD、28.6 kD;病毒粒子包含有25种结构多肽,分子量范围在17.6-114.6 kD之间.PaorNPV DNA经BamH I.EcoR I、HindⅢ、Pst I和Xho I酶切分别产生9、12、12、12和14条片段.基因组大小平均为124.6 kb.     

Influence of cytochrome c on apoptosis induced by Anagrapha (Syngrapha) falcifera multiple nuclear polyhedrosis virus (AfMNPV) in insect Spodoptera litura cells

We investigated the influence of cytochrome c on apoptosis induced by Anagrapha (Syngrapha) falcifera multiple nuclear polyhedrosis virus (AfMNPV). Microscopic observation revealed that infection of SL-1 cells with AfMNPV resulted in apoptosis, displaying apoptotic bodies in fluorescent-stained nuclei of AfMNPV-infected SL-1cells. Western blot analysis demonstrated that AfMNPV-induced apoptosis in insect SL-1 cells was significantly inhibited by cyclosporin A which blocked a translocation of cytochrome c from the mitochondria to the cytosol. As determined by using AC-DEVD-AFC as substrate, the activity of caspase-3 in AfMNPV-induced cells was detected as early as 4h post infection, gradually increased with time extension, and reached a highest level after 16h of infection. However, activity of caspase-3 in apoptotic cells decreased in the presence of cyclosporin A (30microM), indicating that activation of caspase-3 in SfaMNPV-induced cells was dependent on the release of cytochrome c from the mitochondria. In addition, cyclosporin A could markedly inhibit mitochondrial transmembrane potential (DeltaPsim) disruption in undergoing apoptotic cells. These data indicate that cytochrome c plays a key role in AfMNPV-induced apoptosis in S. litura cells and may be required for caspase activation during the induction of apoptosis.     

Some genetic aspects of the resistance of Spodoptera frugiperda to a nuclear polyhedrosis virus

A probit analysis of the dosage-response of two isolates of Spodoptera frugiperda to a single nuclear polyhedrosis virus revealed a greater than 5-fold difference in the LD₅₀. The response of F₁ progeny of reciprocal crosses between the two parental isolates demonstrated that resistance to the virus is not sex-linked. The LD₅₀ values of F₁ and F₂ backcrosses suggest that the major variation in resistance is due to a single gene or genes that lack dominance.     

Electron microscope study on the replication of Autographa nuclear polyhedrosis virus and Spodoptera nuclear polyhedrosis virus in Spodoptera exigua

A comparative study of Spodoptera nuclear polyhedrosis virus (NPV) and Autographa NPV replication in Spodoptera exigua revealed some cytopathologic differences. Infection with Spodoptera NPV was accompanied by electron-dense intranuclear granules. Autographa infection within the midgut led to secretion within the lumens of the goblet cells of paracrystalline arrays of small, round particles, 9.5 nm in diameter. Autographa virus was also observed in various stages of possible replication within the cytoplasm.     

In vivo and in vitro host range of Autographa californica nuclear polyhedrosis virus and Spodoptera frugiperda nuclear polyhedrosis virus

Baculoviruses from Autographa californica (AcNPV-E2) and Spodoptera frugiperda (SfNPV-2) were titered in five insect cell lines: IAL-PID2, IAL-SFD1, IPLB-SF-21AE, TN-368, and IAL-TND1. AcNPV-E2 replicated in all the cell lines while SfNPV-2 did not replicate in the lines TN-368 and IAL-TND1. Further in vivo studies of SfNPV-2 showed the virus was not infectious when fed to Trichoplusia ni larvae per os or when injected into the hemocoel. These data suggest that the barrier to SfNPV-2 infectivity in T. ni is at the cellular level, as opposed to the midgut.     

Host range expansion by recombination of the baculoviruses Bombyx mori nuclear polyhedrosis virus and Autographa californica nuclear polyhedrosis virus.

The mechanisms of host specificity of nuclear polyhedrosis viruses (NPVs) (Baculoviridae) were analyzed after coinfection of Bombyx mori NPV (BmNPV) and one of four distinct groups of Spodoptera litura NPV (SlNPV), including an Autographa californica NPV (AcNPV) variant (S. Maeda, Y. Mukohara, and A. Kondo, J. Gen. Virol. 71:2631-2639, 1990), into various lepidopteran cell lines. Replication of BmNPV in nonpermissive cells (TN-386, SF-21, and CLS-79) was induced by coinfection with AcNPV but not with the other three SlNPV groups. These induced progeny NPVs were plaque purified in BmN cells, which are susceptible to only BmNPV, and characterized. Most of these isolates did not replicate in the cell lines in which they were produced, indicating the existence of a helper function of AcNPV for BmNPV replication in nonpermissive cells. Some of these isolates, however, were able to replicate in cell lines nonpermissive to BmNPV, indicating the appearance of a new virus with wider host specificity. DNA restriction endonuclease analysis showed that the isolates exhibiting wider host range were recombinant viruses between the parents, AcNPV and BmNPV, resulting from various types of crossovers of relatively large areas of their genomes. Expansion of host range was also observed in larvae.     

A nuclear polyhedrosis virus ofHyphantria cunea replicatesin vitro

Summary A nuclear polyhedrosis virus ofHyphantria cunea replicated successfully in theTrichoplusia ni cell line. Restriction endonuclease analysis of the viral DNA obtained from infected cell culture showed the same general homogeneity as that from virus isolated from diseased host larvae. Electron microscopic observations showed that the occluded virus from cell culture consists of rod-like nucleocapsids (31×320 nm) enveloped in aggregates and embedded in polyhedral inclusion bodies from 0.6 to 2.5 m in diameter.     

Polyhedrin gene of Bombyx mori nuclear polyhedrosis virus.

A portion of the genome of the nuclear polyhedrosis virus of Bombyx mori has been cloned. This part of the viral genome contains the gene encoding the viral occlusion body protein, polyhedrin. The polyhedrin gene has been sequenced in its entirety together with some of its 5' and 3' flanking sequences. The primary structure of polyhedrin predicted from the nucleotide sequence of the gene was found to be somewhat different from the one reported previously for the authentic protein (E. A. Kozlov, T. L. Levitina, N. M. Gusak, and S. B. Serebryani, Bioorg. Khim., 7:1008-1015, 1981; S. B. Serebryani, T. L. Levitina, M. L. Kautsman, Y. L. Radavski, N. M. Gusak, M. N. Ovander, N. V. Sucharenko, and E. A. Kozlov, J. Invertebr. Pathol., 30:442-443, 1977). Comparison of the primary structures of the polyhedrin of the nuclear polyhedrosis virus of B. mori with that of Autographa californica suggests that considerable selective pressure has been exercised at the protein level during evolution. Nucleotide sequence comparisons of the two structural genes reveal that the coding sequences have diverged significantly through the accumulation of silent and replacement substitutions. In contrast, a remarkable degree of sequence conservation was found to exist in the domains corresponding to the 5' and 3' noncoding regions of the polyhedrin mRNAs.     

RNP-complex stoichiometry of Bombyx mori nuclear polyhedrosis virus polyhedra

By gel-filtration through Sephacryl S-300 it was shown that RNP A complex present in polyhedra of Bombyx mori nuclear polyhedrosis virus has molecular weight (M(w)) about 700 kDa. It was shown that RNP A with M(w) 788 kDa is composed of two polyhedrin 13S-associates with M(w) 342 kDa, two p14 polypeptide with M(w) 14 kDa, two 21 kDa small non-coded RNAs and two 17 kDa small non-coded RNAs. The model of RNP A formation from components making it is proposed. The complex role in the course of polyhedron formation and its role in the course of infection are discussed.