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.     

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.     

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.     

Food consumption by cabbage loopers infected with nuclear polyhedrosis virus

The effects of age, temperature, and dose on artificial medium consumption by healthy and nuclear polyhedrosis virus-infected cabbage looper larvae were measured using gravimetric methods. Instar in which lethal infection occurred was more closely related to subsequent food consumption than was larval age in days. Larval cabbage loopers, lethally infected in either the first or second instar, consumed 2% or less of their potential consumption. Larvae infected in the third instar consumed ca. 5% of their subsequent potential. In the fourth instar, this amount increased to ca. 10%. If infection occurred in the fifth instar, no significant amount of feeding was prevented. Increasing the virus dosage significantly decreased consumption and length of feeding period over the range of dosages tested. The relationship between consumption patterns of diseased and healthy insects remained constant over a 20–35°C temperature range.     

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.     

Increased virulence of Autographa californica nuclear polyhedrosis virus by mutagenesis

A mutant of the Autographa californica nuclear polyhedrosis virus (AcMNPV) with increased virulence in Trichoplusia ni larvae was isolated following replication of a random virus clone in the presence of 2-aminopurine. The LT₅₀ of the mutant, designated HOB, was significantly shorter than those of either the wild isolate or parental clone of AcMNPV. Also, fifth-instar larvae infected with this mutant gained significantly less weight and consistently produced more virus occlusion bodies than larvae infected with the wild isolate or parental clone. No alterations in the in vitro replication of nonoccluded virions, occluded virus structural proteins, or DNA restriction endonuclease patterns were observed with the HOB mutant.     

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.     

Infectivity of nuclear polyhedrosis virus extracted with digestive juices

Autographa californica NPV, which had been obtained by dissolving polyhedra in the digestive juice of Estigmene acrea larvae, was infectious to a Trichoplusia ni cell line (TN-368). Virions thus botained were infective, and as few as 0.0025–0.005 polyhedral equivalents could infect newly transferred tissue culture cells. Activity decreased after 8 min of digestion.     

芹菜夜蛾核型多角体病毒D克隆株某些理化性质的研究

杆状病毒由于其专一致死宿主昆虫、对人畜无害、无环境残留、害虫不易产生抗性等优点,广泛用于农林有害昆虫的防治,但杆状病毒杀虫剂也具有杀虫谱窄、杀虫速度慢等缺点.后来科学家先后发现了广谱毒株——苜蓿银纹夜蛾核型多角体病毒(Autographa californica nuclear polyhedrosis virus AcNPV)、芹菜夜蛾核型多角体病毒(Syngrapha falcifera nuclear polyhedrosis virus SfaNPV),可感染磷翅目三十多种昆虫,前者对已产生农药抗性的常见农业害虫小菜蛾、棉铃虫不敏感,而后者对它们有较高毒力[1～3].我们实验室通过空斑纯化技术得到 Sfa- D 克隆株,此毒株对多种农业害虫具有很强的毒力.本文对该毒株的理化性质做了较为详细的研究,以期为该株病毒的利用提供理论依据.     

Safety evaluation of nuclear polyhedrosis virus replication in pigs

To evaluate the hygienic risk involved in using baculoviruses for insect pest control, safety studies are required. Pigs were chosen as representative test animals of commercial and agricultural importance. The tests were aimed at detecting virus propagation, immune reactions, and signs of acute infection (changes in body temperature and hematology profile, swelling of lymph nodes). Four of five animals inoculated with nuclear polyhedrosis virus showed a slight temperature rise at day 2 postinfection. After day 4 postinfection, no differences between infected animals and controls were observed. In the bioassay, virus activity could be recovered from fecal samples; however, no activity was found in organ extracts. The data did not indicate hygienic risks involved in the application of nuclear polyhedrosis virus, especially that from Mamestra brassicae, in biological pest control.     

Safety evaluation of nuclear polyhedrosis virus replication in pigs.

To evaluate the hygienic risk involved in using baculoviruses for insect pest control, safety studies are required. Pigs were chosen as representative test animals of commercial and agricultural importance. The tests were aimed at detecting virus propagation, immune reactions, and signs of acute infection (changes in body temperature and hematology profile, swelling of lymph nodes). Four of five animals inoculated with nuclear polyhedrosis virus showed a slight temperature rise at day 2 postinfection. After day 4 postinfection, no differences between infected animals and controls were observed. In the bioassay, virus activity could be recovered from fecal samples; however, no activity was found in organ extracts. The data did not indicate hygienic risks involved in the application of nuclear polyhedrosis virus, especially that from Mamestra brassicae, in biological pest control.