In vitro cultivation of Wolbachia in insect and mammalian cell lines

Wolbachia infecting the small brown planthopper, Laodelphax striatellus, were successfully maintained and cultivated in two insect and one mammalian cell lines. The bacteria with the planthopper ovary were introduced into the flasks with the cultures of the cell lines. The Wolbachia proliferated in mosquito (Aedes albopictus) and lepidopteran (Heliothis zea) cell lines and in the mouse cell line, L929. Proliferation of Wolbachia was confirmed by electron microscopy and quantitative polymerase chain reaction. This simple method for the cultivation of Wolbachia was applicable to other strains of Wolbachia, such as the one found in the lepidopteran eggs, and should facilitate fundamental and applied studies of this important group of microorganisms.     

Specificity of Bacillus thuringiensis var. colmeri insecticidal delta-endotoxin is determined by differential proteolytic processing of the protoxin by larval gut proteases

The native crystal delta-endotoxin produced by Bacillus thuringiensis var. colmeri, serotype 21, is toxic to both lepidopteran (Pieris brassicae) and dipteran (Aedes aegypti) larvae. Solubilization of the crystal delta-endotoxin in alkaline reducing conditions and activation with trypsin and gut extracts from susceptible insects yielded a preparation whose toxicity could be assayed in vitro against a range of insect cell lines. After activation with Aedes aegypti gut extract the preparation was toxic to all of the mosquito cell lines but only one lepidopteran line (Spodoptera frugiperda), whereas an activated preparation produced by treatment with P. brassicae gut enzymes or trypsin was toxic only to lepidopteran cell lines. These in vitro results were paralleled by the results of in vivo bioassays. Gel electrophoretic analysis of the products of these different activation regimes suggested that a 130-kDa protoxin in the native crystal is converted to a 55-kDa lepidopteran-specific toxin by trypsin or P. brassicae enzymes and to a 52-kDa dipteran toxin by A. aegypti enzymes. Two-step activation of the 130-kDa protoxin by successive treatment with trypsin and A. aegypti enzymes further suggested that the 52-kDa dipteran toxin is derived from the 55-kDa lepidopteran toxin by enzymes specific to the mosquito gut. Confirmation of this suggestion was obtained by peptide mapping of these two polypeptides. The native crystal 130 kDa delta-endotoxin and the two insect-specific toxins all cross-reacted with antiserum to B. thuringiensis var. kurstaki P1 lepidopteran toxin. Preincubation of the two activated colmeri toxins with P1 antiserum neutralized their cytotoxicity to both lepidopteran and dipteran cell lines.     

Characterization of invertebrate cell lines

Summary The usefulness of four serologic techniques for distinguishing five selected lepidopteran cell lines was evaluated; the techniques included complement fixation, hemagglutination. immunodiffusion, and immunoelectrophoresis. The five selected lepidopteran cell lines represent three taxonomic families of Lepidoptera with one family, Noctuidae, containing two cell lines derived from insects within the same genus. The five cell lines were crossreactive in complement-fixation tests, but the lines were distinguishable at a familic level when two units of antigens were used in the test. Agglutination of goose erythrocytes was not observed with the antigens over a pH range of 5.8 to 7.2 at 4°C or ambient temperature. Immunodiffusion tests demonstrated a common cross-reactive antigen(s), but spurs of partial identity and the presence of extra precipitin bands were indicative that differentiation at a familic level was possible. Immunoelectrophoresis of the cellular antigens also revealed common cross-reactive precipitin arcs, but the number and clarity of arcs in homologous systems was increased such that four of the five cell lines were distinguishable. A basic protein was consistently seen in the homologous system, but it was absent in the heterologous systems. Although these data suggest that immunoelectrophoresis was the best serologic technique for distinguishing the five lepidopteran cell lines, the shortcomings of this approach are also discussed. This research was supported in part by the World Health Organization, The Rockefeller Foundation, and U.S. Public Health Service Grant AI-13727.     

Diversity of G proteins in Lepidopteran cell lines: partial sequences of six G protein alpha subunits

The aim of this work was to sample the diversity of G protein alpha subunits in lepidopteran insect cell lines. Here we report the amplification by degenerate PCR of partial sequences representing six G protein alpha subunits from three different lepidopteran insect cell lines. Sequence comparisons with known G protein alpha subunits indicate that the Sf9, Ld and High Five cell lines each contain (at least) one Galpha(q)-like and one Galpha(i)-like Galpha subunit. All six PCR products are unique at the nucleotide level, but the translation products of the three Galpha q-like partial clones (Sf9-Galpha 1, Ld-Galpha 1, and Hi5-Galpha 1) are identical, as are the translation products of the three Galpha i-like partial clones (Sf9-Galpha 2, Ld-Galpha 2, and Hi5-Galpha 2). Both the Galpha(q)-like and Galpha(i)-like translation products are identical to known Galpha subunits from other Lepidoptera, are highly similar (88-98%) to Galpha subunits from other invertebrates including mosquitoes, fruit flies, lobsters, crabs, and snails, and are also highly similar (88-90%) to known mammalian Galpha subunits. Identification of G protein alpha subunits in lepidopteran cell lines will assist in host cell line selection when insect cell lines are used for the pharmacological analysis of human GPCRs.     

Establishment and characterization of a continuous cell line from pupal ovaries of Japanese oak silkworm Antheraea yamamai Guerin-Meneville

Pupal ovaries of the wild oak silkworm Antheraea yamamai Guerin-Meneville were cultured in MGM-448 (Modified Grace Medium-448) medium containing 10% fetal bovine serum. After the primary culture was set up in 1988, a continuous cell line was obtained in 1991, designated as NISES-Anya-0611 (Anya-0611). The population doubling time was 54 hrs. and 19 min. at 96 passages and 88 hrs. and 29 min. at 387 passages. Spindle-shaped and spherical cells coexisted in the cell group. The cell line karyotype line was typical of lepidopteran cell lines, consisting of numerous small chromosomes. The cell line was distinguished from other lepidopteran cell lines by comparing malic enzyme, phosphoglucose isomerase, phosphoglucose mutase, and isocitric dehydrogenase isozyme patterns. The cell line was highly infected to the Antheraea yamamai nuclear polyhedrosis virus (Anya NPV). The luciferase gene of recombinant Bm NPV (BmNPVP6ETL) was able to express in the cell line, too, so that luciferase recombinant products were able to be detected in the cell body and in supernatant. The Anya NPV clone group was isolated on the cell seat using plaque purification.     

新细胞系──粘虫胚胎细胞系的建立(英文)

一株新细胞系-粘虫（Mythimnaseparata）胚胎细胞系（NEAU－Ms－927311简称Ms937311）被建立。该细胞系多为梭形细胞,少数圆形,贴壁性强。细胞群体倍增时间为58．8h;接种3天后细胞增长速度加快,第5天达到最大值;染色体分析结果表明：染色体聚集成簇,棒球状,呈典型的鳞翅目昆虫细胞核型;酯酶同工酶分析有两条明显的谱带;该细胞系可被同源核型多角体病毒（MsNPV）侵染并形成多角体。     

NEW CELL LINE FROM EMBRYOS OF MYTHIMNA SEPARATA (LEPIDOPTERA: NOCTUIDAE)

Abstract  A new cell line was established from 2-d-old embryonated eggs of Mythimna separata and has been designated as NEAU-Ms-927311. This cell line consists of a mixture of cell types, including spherical and spindle-shaped cells. The cell line has a population doubling time of 58. 8h. Chromosome analysis revealed its typical lepidopteran karyology. Isozyme characterization of esterase showed that the band pattern was different from that of other two cell lines (Xc-920730, and SF-21AE). Virus infectivity tests revealed this cell line can support replication of M. separata nuclear polyhedrosis virus.     

Establishment of a cell line from embryos of the cabbage looper,Trichoplusia ni (hubner)

Summary A new cell line was developed from 3-d-old embryonated eggs of the cabbage looper,Trichoplusia ni, and has been designated IPLB-TN-R². It contains a variety of morphological cell types, including myoblastlike, neuroblastlike, and epithelial-like cells. Chromosome analysis revealed typical lepidopteran chromosomes. Isozyme characterization showed patterns similar to two other cabbage looper cell lines (TN-368 and IAL-TND1) in the case of five enzymes but differed from these two lines for two other enzymes. Virus infectivity tests revealed the line is highly susceptible toAutographa californica nuclear polyhedrosis virus, but no cytopathology was observed after inoculation with several other lepidopteran viruses.     

Application of inter-simple sequence repeats to insect cell lines: identification at the clonal and tissue-specific level

Inter-simple sequence repeat (ISSR) primers designed to anneal to microsatellites were used to obtain deoxyribonucleic acid (DNA) fingerprint profiles to distinguish among 16 established insect cell lines derived from an assortment of lepidopteran, dipteran, and coleopteran species. Three different levels of cell line comparison were made: (1) between parents and their clones, (2) among cell lines derived from different tissues from the same species, and (3) among cell lines derived from different insect species. Of the 16 repeat oligonucleotide primers used in this study, nine primers generated several unique markers to distinguish between parental cell lines and their clones. Four of the 16 primers also generated DNA profiles with a number of unique bands, enabling the distinction among cell lines derived from specific tissues from the same species. In addition, ISSR-generated DNA profiles provided the greatest number of unique markers to distinguish easily among insect cell lines derived from different species.     

八字地老虎血球细胞系的建立

由八字地老虎Xestia c-nigrum血细胞建立了一株细胞系,命名为NEAU-Xc-960716H,原代培养90余天,现已传至70余代。细胞多为圆形,部分梭形,细胞群体倍增时间约为63 h。具有典型的鳞翅目昆虫染色体特征,数量多,形态为短杆状和球形。酯酶同工酶谱为5条主带,与同种昆虫（八字地老虎）的胚胎细胞系(NEAU-Xc-730E)酯酶图谱稍有不同,而与草地夜蛾细胞系(IPLB-SF-21)的酯酶图谱完全不同。该细胞系可以被八字地老虎核型多角体病毒XcNPV感染,但感染率较低。