Your search keyword '"Insect Proteins biosynthesis"' showing total 666 results

101. Expression and characterization of a fibrinogenolytic enzyme from horsefly salivary gland.

Author

Sheng X, Gao L, Lu X, Wang Y, Han Y, Meng P, Chen W, and Lu Q

Subjects

Animals, Diptera enzymology, Humans, Insect Proteins biosynthesis, Insect Proteins chemistry, Insect Proteins genetics, Insect Proteins isolation & purification, Recombinant Proteins, Salivary Proteins and Peptides biosynthesis, Salivary Proteins and Peptides genetics, Salivary Proteins and Peptides isolation & purification, Diptera genetics, Fibrinolytic Agents chemistry, Fibrinolytic Agents isolation & purification, Fibrinolytic Agents metabolism, Salivary Glands

Abstract

Enzymes from various natural resources are valuable in management of thrombosis. Blood-sucking arthropods are one of these resources because they have a wide array of anti-hemostasis molecules in their salivary gland. However, it is difficult to purify enough protein samples from the salivary glands for pharmacological studies. In this work, a fibrinogenolytic enzyme (tablysin 2) identified from salivary glands of the horsefly Tabanus yao was expressed in Escherichia coli to further study its biological activities. The primary structure of tablysin 2 showed significant domain similarity to arthropod proteins from the antigen 5 family containing SCP domain, whose biological functions are poorly understood. Tablysin 2 cleaved the Aα and part of Bβ chains of fibrinogen and did not affect γ chain and fibrin. It inhibited platelet aggregation induced by ADP. It did not directly induce hemorrhage or activate plasminogen. The fibrinogenolytic activity of tablysin 2 provides a clue for the functions of antigen 5-related proteins in other haematophagous arthropods. This work demonstrate a method of expression of arthropod salivary proteins which are difficult to obtain from natural resources for further functional studies., (Copyright © 2016 Elsevier Inc. All rights reserved.)

Published

2017

102. Characterization and Expression Analysis of Attacins, Antimicrobial Peptide-Encoding Genes, from the Desert Beetle Microdera punctipennis in Response to Low Temperatures.

Author

Li JQ, Lu XY, and Ma J

Subjects

Amino Acid Sequence, Animals, Cold Temperature, Gene Expression Regulation physiology, Molecular Sequence Data, Phylogeny, Real-Time Polymerase Chain Reaction, Temperature, Adaptation, Physiological physiology, Coleoptera physiology, Insect Proteins biosynthesis

Abstract

Background: Antimicrobial peptides (AMPs) constitute the insect innate immune defense system. AMP production is usually induced by microbes. However, mounting evidence links insect immune reaction to cold hardiness., Objective: We aimed at characterizing two attacins, MpAtt1 and MpAtt2, from the desert beetle Microdera punctipennis in Coleoptera and investigating the expression profiles of the two genes in response to cold stress., Results: Full lengths MpAtt1 and MpAtt2 cDNAs were obtained from low temperature transcriptomic data. The newly identified attacins show characteristics different from those previously reported in other insects. MpAtt1 and MpAtt2 encode precursor proteins of 151 and 166 amino acid residues, respectively. These two attacins show 28.1% identity at amino acid level, and 38.3% identity at nucleotide level. Phylogenetic tree shows that the Mp attacins and the other Coleoptera attacins diverge earlier than Diptera and Lepidoptera attacins in evolution. The results of real-time quantitative PCR showed that MpAtt1 and MpAtt2 are highly expressed in hindgut plus Malpighian tube, and MpAtt1 also highly expressed in fat body. The mRNA levels of MpAtt1 and MpAtt2 were increased when the insects were treated at 4 degree C and a4 degree C, but the responsiveness to -4 degree C was lower than to 4 degree C., Conclusion: The cold inducible expression of attacin genes from the desert beetle M. punctipennis from the aspect of antimicrobial peptide synthesis supports the hypothesis that the insect immune system is stimulated during cold exposure.

Published

2017

103. Nitric oxide synthase during early embryonic development in silkworm Bombyx mori: Gene expression, enzyme activity, and tissue distribution.

Author

Kitta R, Kuwamoto M, Yamahama Y, Mase K, and Sawada H

Subjects

Animals, Bombyx embryology, Organ Specificity physiology, Bombyx enzymology, Embryonic Development physiology, Gene Expression Regulation, Developmental physiology, Gene Expression Regulation, Enzymologic physiology, Insect Proteins biosynthesis, Nitric Oxide Synthase biosynthesis

Abstract

To elucidate the mechanism for embryonic diapause or the breakdown of diapause in Bombyx mori, we biochemically analyzed nitric oxide synthase (NOS) during the embryogenesis of B. mori. The gene expression and enzyme activity of B. mori NOS (BmNOS) were examined in diapause, non-diapause, and HCl-treated diapause eggs. In the case of HCl-treated diapause eggs, the gene expression and enzyme activity of BmNOS were induced by HCl treatment. However, in the case of diapause and non-diapause eggs during embryogenesis, changes in the BmNOS activity and gene expressions did not coincide except 48-60 h after oviposition in diapause eggs. The results imply that changes in BmNOS activity during the embryogenesis of diapause and non-diapause eggs are regulated not only at the level of transcription but also post-transcription. The distribution and localization of BmNOS were also investigated with an immunohistochemical technique using antibodies against the universal NOS; the localization of BmNOS was observed mainly in the cytoplasm of yolk cells in diapause eggs and HCl-treated diapause eggs. These data suggest that BmNOS has an important role in the early embryonic development of the B. mori., (© 2016 Japanese Society of Developmental Biologists.)

Published

2016

104. Helicoidal Organization of Chitin in the Cuticle of the Migratory Locust Requires the Function of the Chitin Deacetylase2 Enzyme (LmCDA2).

Author

Yu R, Liu W, Li D, Zhao X, Ding G, Zhang M, Ma E, Zhu K, Li S, Moussian B, and Zhang J

Subjects

Amidohydrolases genetics, Animals, Chitin genetics, Insect Proteins genetics, Locusta migratoria genetics, Amidohydrolases biosynthesis, Chitin metabolism, Gene Expression Regulation, Enzymologic physiology, Insect Proteins biosynthesis, Locusta migratoria enzymology, Molting physiology

Abstract

In the three-dimensional extracellular matrix of the insect cuticle, horizontally aligned microfibrils composed of the polysaccharide chitin and associated proteins are stacked either parallel to each other or helicoidally. The underlying molecular mechanisms that implement differential chitin organization are largely unknown. To learn more about cuticle organization, we sought to study the role of chitin deacetylases (CDA) in this process. In the body cuticle of nymphs of the migratory locust Locusta migratoria, helicoidal chitin organization is changed to an organization with unidirectional microfibril orientation when LmCDA2 expression is knocked down by RNA interference. In addition, the LmCDA2-deficient cuticle is less compact suggesting that LmCDA2 is needed for chitin packaging. Animals with reduced LmCDA2 activity die at molting, underlining that correct chitin organization is essential for survival. Interestingly, we find that LmCDA2 localizes only to the initially produced chitin microfibrils that constitute the apical site of the chitin stack. Based on our data, we hypothesize that LmCDA2-mediated chitin deacetylation at the beginning of chitin production is a decisive reaction that triggers helicoidal arrangement of subsequently assembled chitin-protein microfibrils., (© 2016 by The American Society for Biochemistry and Molecular Biology, Inc.)

Published

2016

105. Comparative RNA-sequencing profiling reveals novel Delta-class glutathione S-transferases relative genes expression patterns in Tribolium castaneum.

Author

Chen X, Xiong W, Li C, Gao S, Song X, Wu W, and Li B

Subjects

Animals, Gene Expression Profiling, High-Throughput Nucleotide Sequencing, Gene Expression Regulation, Enzymologic physiology, Glutathione Transferase biosynthesis, Glutathione Transferase genetics, Insect Proteins biosynthesis, Insect Proteins genetics, Tribolium enzymology, Tribolium genetics

Abstract

Glutathione S-transferases (GSTs) are a large group of enzymes having both detoxification roles conferring insecticide resistance and specialist metabolic functions. Tribolium castaneum GST Delta 1 (TcGSTd1) has been found playing crucial role in insecticide resistance and biological processes in insect species. However, the regulatory system of TcGSTd1 has still rarely been known. Comparing the transcriptome profile of RNAi treated larvae (ds-TcGSTd1) and control larvae of T. canstaneum by using RNA-sequencing, we obtained 14,284,085 sequence reads aligned with 13,275 genes. And 512 differentially expressed genes (DEGs) were identified from ds-TcGSTd1 treated group. Est/CCE, CYP, MRPs were significantly down-regulated in ds-TcGSTd1 group when compared with control group, which illustrated that they cooperated with TcGSTd1 to reduce the activity of cellular metabolism system. While, SNO was up-regulated in ds-TcGSTd1 insects suggested it may also involve in detoxifying alkaloid of insect metabolism system. These results established that TcGSTd1 not only acts as a vital gene for phase II cellular detoxification but also participates in phase 0, I, and III cellular detoxification by cooperating with CSPs, OBPs, CYP9, ESTB1, CCE6, MRPs and other detoxification genes. Knockdown of TcGSTd1 also suppressed several genes encoding antioxidant enzymes, e.g. CuZnSOD, Duox, Prx, HPX, CPO, and MCORP. Suggested that they may modulate the function of TcGSTd1 on lifespan, immune, development and reproduction. All these results shed the new insights into the regulatory mechanism of TcGSTd1 involved in insect physiology and could further facilitate the research of suitable and sustainable managements for the pest control., (Copyright © 2016 Elsevier B.V. All rights reserved.)

Published

2016

106. Type III secretion as a generalizable strategy for the production of full-length biopolymer-forming proteins.

Author

Azam A, Li C, Metcalf KJ, and Tullman-Ercek D

Subjects

Recombinant Proteins genetics, Insect Proteins biosynthesis, Insect Proteins genetics, Protein Engineering methods, Recombinant Proteins biosynthesis, Salmonella enterica physiology, Type III Secretion Systems physiology

Abstract

Biopolymer-forming proteins are integral in the development of customizable biomaterials, but recombinant expression of these proteins is challenging. In particular, biopolymer-forming proteins have repetitive, glycine-rich domains and, like many heterologously expressed proteins, are prone to incomplete translation, aggregation, and proteolytic degradation in the production host. This necessitates tailored purification processes to isolate each full-length protein of interest from the truncated forms as well as other contaminating proteins; owing to the repetitive nature of these proteins, the truncated polypeptides can have very similar chemistry to the full-length form and are difficult to separate from the full-length protein. We hypothesized that bacterial expression and secretion would be a promising alternative option for biomaterials-forming proteins, simplifying isolation of the full-length target protein. By using a selective secretion system, truncated forms of the protein are not secreted and thus are not found in the culture harvest. We show that a synthetically upregulated type III secretion system leads to a general increase in secretion titer for each protein that we tested. Moreover, we observe a substantial enhancement in the homogeneity of full-length forms of pro-resilin, tropo-elastin crosslinking domains, and silk proteins produced in this manner, as compared with proteins purified from the cytosol. Secretion via the type III apparatus limits co-purification of truncated forms of the target protein and increases protein purity without extensive purification steps. Demonstrating the utility of such a system, we introduce several modifications to resilin-based peptides and use an un-optimized, single-column process to purify these proteins. The resulting materials are of sufficiently high quantity and yield for the production of antimicrobial hydrogels with highly reproducible rheological properties. The ease of this process and its applicability to an array of engineered biomaterial-forming peptides lend support for the application of bacterial expression and secretion for other proteins that are traditionally difficult to express and isolate from the bacterial cytoplasm. Biotechnol. Bioeng. 2016;113: 2313-2320. © 2015 Wiley Periodicals, Inc., (© 2015 Wiley Periodicals, Inc.)

Published

2016

107. [Cloning and expression of scavenger receptor class B BmSCRB8 in silkworm Bombyx mori].

Author

Zhao Y, Zhang K, Tang M, Xu M, Li C, Pan G, Shen L, Cui H, and Yang L

Subjects

Amino Acid Sequence, Animals, Base Sequence, Cloning, Molecular, DNA, Complementary, Bombyx, Insect Proteins biosynthesis, Receptors, Scavenger biosynthesis

Abstract

Scavenger receptor class B is involved in various indispensable physiological processes, like the formation and inhibition of atherosclerosis or other cardiovascular diseases, innate immune defense and the removal of apoptotic cells. Here, we cloned BmSCRB8, a member of scavenger receptor class B in silkworm. We obtained the full-length cDNA sequence of BmSCRB8 by rapid amplification of cDNA ends (RACE), including 2 668 bp. The ORF of BmSCRB8 is 1 704 bp, encoding 567 amino acids. Online software prediction indicated that the molecular weight of BmSCRB8 is 63.87 kDa and the isoelectric point (pI) is 6.06. The space-time expression profile of BmSCRB8 was detected by reverse transcription PCR (RT-PCR), which implicated that BmSCRB8 is extensively expressed in each tissue and at each stage of blood. In addition, BmSCRB8 is highest expressed in fat body of silkworm, and is highly expressed in metamorphosis periods. Anti-BmSCRB8 polyclonal antibody was generated through prokaryotic expression, protein purification and mice immunization. Simultaneously, we constructed BmSCRB8 eukaryotic vector and then transfected embryonic cell line of silkworm. Immunofluorescence and overexpression showed that BmSCRB8 expressed specifically in membrane. Western blotting demonstrated that BmSCRB8 protein can be specifically recognized by anti-serum generated after mice immunization.

Published

2016

108. [Soluble expression, purification and structural analysis of the bHLH transcription factor Bmsage of Bombyx mori].

Author

He H, Wei S, Wang Y, Liu L, Li Z, Zhao P, Chang H, and Zhao P

Subjects

Animals, Basic Helix-Loop-Helix Transcription Factors chemistry, Escherichia coli, Insect Proteins chemistry, Protein Structure, Secondary, Silk, Basic Helix-Loop-Helix Transcription Factors biosynthesis, Bombyx, Insect Proteins biosynthesis

Abstract

Basic helix loop helix (bHLH) transcription factor plays an important role in biological processes. Bmsage is a class of bHLH transcription factor highly expressed in the silk gland of Bombyx mori, which is not only involved in the developmental regulation of the silk gland cells at the embryonic period, but also plays a crucial regulatory role during the synthesis of silk protein. However, currently, much of the property and structure of Bmsage is still remained unknown. To study the property, structure and biological role of Bmsage, we constructed several prokaryotic expression vectors of Bmsage fused with NusA, MBP, SUMO, Trx and His tags, respectively, then screened and determined the best soluble expression vector and condition of Bmsage in Escherichia coli combining with the induction temperature and IPTG concentration, and further purified the recombinant Bmsage by Ni-column affinity chromatography according to the established expression condition and characterized its secondary structure using circular dichroism spectra. The results showed that NusA and MBP could significantly enhance the soluble expression of Bmsage in E. coli, but it was difficult to separate Bmsage from these tags. SUMO could not only increase the soluble expression of Bmsage in E. coli to a certain degree, but also be effectively separated from Bmsage. Other tags did not effectively promote the soluble expression of Bmsage in E. coli. Circular dichroism spectra showed that the purified Bmsage had well-defined α-helix structure in solution, indicating that SUMO may promote the correct folding of Bmsage into native-like structure. These work not only establish a foundation for further study of the property, structure and function of Bmsage, but also provide a reference for the expression and purification of other similar proteins.

Published

2016

109. 35S Promoter Methylation in Kanamycin-Resistant Kalanchoe (Kalanchoe pinnata L.) Plants Expressing the Antimicrobial Peptide Cecropin P1 Transgene.

Author

Shevchuk TV, Zakharchenko NS, Tarlachkov SV, Furs OV, Dyachenko OV, and Buryanov YI

Subjects

DNA Methylation, DNA, Plant genetics, DNA, Plant metabolism, Drug Resistance, Insect Proteins biosynthesis, Insect Proteins genetics, Kalanchoe genetics, Kalanchoe metabolism, Kanamycin, Plants, Genetically Modified genetics, Plants, Genetically Modified metabolism, Promoter Regions, Genetic, Transgenes

Abstract

Transgenic kalanchoe plants (Kalanchoe pinnata L.) expressing the antimicrobial peptide cecropin P1 gene (cecP1) under the control of the 35S cauliflower mosaic virus 35S RNA promoter and the selective neomycin phosphotransferase II (nptII) gene under the control of the nopaline synthase gene promoter were studied. The 35S promoter methylation and the cecropin P1 biosynthesis levels were compared in plants growing on media with and without kanamycin. The low level of active 35S promoter methylation further decreases upon cultivation on kanamycin-containing medium, while cecropin P1 synthesis increases.

Published

2016

110. Synthesis and biological activity of FGLamide allatostatin analogs with Phe(3) residue modifications.

Author

Xie Y, Wang M, Zhang L, Wu X, Yang X, and Tobe SS

Subjects

Amino Acid Sequence, Animals, Cockroaches drug effects, Cockroaches genetics, Cockroaches metabolism, Corpora Allata metabolism, Dose-Response Relationship, Drug, Female, Gene Expression Regulation, Hormone Antagonists pharmacology, Insect Proteins biosynthesis, Insect Proteins genetics, Juvenile Hormones biosynthesis, Juvenile Hormones genetics, Male, Neuropeptides pharmacology, Peptidomimetics pharmacology, Phenylalanine chemistry, Phenylalanine metabolism, Structure-Activity Relationship, Corpora Allata drug effects, Hormone Antagonists chemical synthesis, Insect Proteins antagonists & inhibitors, Juvenile Hormones antagonists & inhibitors, Neuropeptides chemical synthesis, Peptidomimetics chemical synthesis

Abstract

A FGLamide allatostatin neuropeptide mimic (H17) is a potential insect growth regulator which inhibits the production of juvenile hormone by the corpora allata. To find more evidence to reveal the structure-activity relationships of the Phe(3) residue in the C-terminal conserved pentapeptide and search for novel analogs with high activity, a series of Phe(3) residue-modified analogs were designed and synthesized using H17 as the lead compound. Bioassay using juvenile hormone (JH) production by corpora allata of the cockroach Diploptera punctata indicated that analogs 4, 11, and 13 showed strong ability to inhibit JH production in vitro, with IC50 of 38.5, 22.5, and 26 nM, respectively. As well, the activity of analog 2 (IC50 : 89.5 nM) proved roughly equivalent to that of H17. Based on the primary structure-activity relationships of Phe(3) residue, we suggest that for analogs containing six-membered aromatic rings, removing the methylene group of Phe(3) or an o-halogen or p-halogen-substituted benzene ring could increase the ability to inhibit biosynthesis of JH. This study will be useful for the design of new allatostatin analogs for insect management. Copyright © 2016 European Peptide Society and John Wiley & Sons, Ltd., (Copyright © 2016 European Peptide Society and John Wiley & Sons, Ltd.)

Published

2016

111. Differential expression of genes in the alate and apterous morphs of the brown citrus aphid, Toxoptera citricida.

Author

Shang F, Ding BY, Xiong Y, Dou W, Wei D, Jiang HB, Wei DD, and Wang JJ

Subjects

Animals, Aphids anatomy & histology, Aphids growth & development, Aphids metabolism, Energy Metabolism genetics, Gene Expression Profiling, Insect Proteins genetics, Lipid Metabolism genetics, Molecular Sequence Annotation, RNA, Messenger biosynthesis, RNA, Messenger genetics, Sequence Analysis, RNA, Transcriptome, Wings, Animal metabolism, Aphids genetics, Gene Expression Regulation, Genes, Insect, Insect Proteins biosynthesis, Metabolic Networks and Pathways genetics, Wings, Animal growth & development

Abstract

Winged and wingless morphs in insects represent a trade-off between dispersal ability and reproduction. We studied key genes associated with apterous and alate morphs in Toxoptera citricida (Kirkaldy) using RNAseq, digital gene expression (DGE) profiling, and RNA interference. The de novo assembly of the transcriptome was obtained through Illumina short-read sequencing technology. A total of 44,199 unigenes were generated and 27,640 were annotated. The transcriptomic differences between alate and apterous adults indicated that 279 unigenes were highly expressed in alate adults, whereas 5,470 were expressed at low levels. Expression patterns of the top 10 highly expressed genes in alate adults agreed with wing bud development trends. Silencing of the lipid synthesis and degradation gene (3-ketoacyl-CoA thiolase, mitochondrial-like) and glycogen genes (Phosphoenolpyruvate carboxykinase [GTP]-like and Glycogen phosphorylase-like isoform 2) resulted in underdeveloped wings. This suggests that both lipid and glycogen metabolism provide energy for aphid wing development. The large number of sequences and expression data produced from the transcriptome and DGE sequencing, respectively, increases our understanding of wing development mechanisms.

Published

2016

112. Transgenic Expression of the piRNA-Resistant Masculinizer Gene Induces Female-Specific Lethality and Partial Female-to-Male Sex Reversal in the Silkworm, Bombyx mori.

Author

Sakai H, Sumitani M, Chikami Y, Yahata K, Uchino K, Kiuchi T, Katsuma S, Aoki F, Sezutsu H, and Suzuki MG

Subjects

Animals, Animals, Genetically Modified, Bombyx growth & development, DNA-Binding Proteins biosynthesis, Female, Gene Expression Regulation, Developmental, Insect Proteins biosynthesis, Insulin-Like Growth Factor II biosynthesis, Male, Ovary growth & development, Ovary metabolism, RNA Splicing genetics, RNA, Small Interfering biosynthesis, Sex Chromosomes genetics, Testis growth & development, Testis metabolism, Vitellogenins biosynthesis, Vitellogenins genetics, Bombyx genetics, DNA-Binding Proteins genetics, Insect Proteins genetics, Insulin-Like Growth Factor II genetics, RNA, Small Interfering genetics, Sex Determination Processes genetics

Abstract

In Bombyx mori (B. mori), Fem piRNA originates from the W chromosome and is responsible for femaleness. The Fem piRNA-PIWI complex targets and cleaves mRNAs transcribed from the Masc gene. Masc encodes a novel CCCH type zinc-finger protein and is required for male-specific splicing of B. mori doublesex (Bmdsx) transcripts. In the present study, several silkworm strains carrying a transgene, which encodes a Fem piRNA-resistant Masc mRNA (Masc-R), were generated. Forced expression of the Masc-R transgene caused female-specific lethality during the larval stages. One of the Masc-R strains weakly expressed Masc-R in various tissues. Females heterozygous for the transgene expressed male-specific isoform of the Bombyx homolog of insulin-like growth factor II mRNA-binding protein (ImpM) and Bmdsx. All examined females showed a lower inducibility of vitellogenin synthesis and exhibited abnormalities in the ovaries. Testis-like tissues were observed in abnormal ovaries and, notably, the tissues contained considerable numbers of sperm bundles. Homozygous expression of the transgene resulted in formation of the male-specific abdominal segment in adult females and caused partial male differentiation in female genitalia. These results strongly suggest that Masc is an important regulatory gene of maleness in B. mori., Competing Interests: The authors have declared that no competing interests exist.

Published

2016

113. 20-Hydroxyecdysone (20E) Primary Response Gene E75 Isoforms Mediate Steroidogenesis Autoregulation and Regulate Developmental Timing in Bombyx.

Author

Li K, Tian L, Guo Z, Guo S, Zhang J, Gu SH, Palli SR, Cao Y, and Li S

Subjects

Animals, Bombyx genetics, Ecdysterone genetics, Insect Proteins genetics, Protein Isoforms, Bombyx embryology, Ecdysterone metabolism, Gene Expression Regulation, Developmental physiology, Genes, Insect physiology, Insect Proteins biosynthesis, Metamorphosis, Biological physiology

Abstract

The temporal control mechanisms that precisely control animal development remain largely elusive. The timing of major developmental transitions in insects, including molting and metamorphosis, is coordinated by the steroid hormone 20-hydroxyecdysone (20E). 20E involves feedback loops to maintain pulses of ecdysteroid biosynthesis leading to its upsurge, whereas the underpinning molecular mechanisms are not well understood. Using the silkworm Bombyx mori as a model, we demonstrated that E75, the 20E primary response gene, mediates a regulatory loop between ecdysteroid biosynthesis and 20E signaling. E75 isoforms A and C directly bind to retinoic acid receptor-related response elements in Halloween gene promoter regions to induce gene expression thus promoting ecdysteroid biosynthesis and developmental transition, whereas isoform B antagonizes the transcriptional activity of isoform A/C through physical interaction. As the expression of E75 isoforms is differentially induced by 20E, the E75-mediated regulatory loop represents a fine autoregulation of steroidogenesis, which contributes to the precise control of developmental timing., (© 2016 by The American Society for Biochemistry and Molecular Biology, Inc.)

Published

2016

114. Microbial production of amino acid-modified spider dragline silk protein with intensively improved mechanical properties.

Author

Zhang H, Zhou F, Jiang X, Cao M, Wang S, Zou H, Cao Y, Xian M, and Liu H

Subjects

Amino Acid Sequence, Animals, Disulfides chemistry, Elasticity, Fermentation, Insect Proteins chemistry, Insect Proteins metabolism, Microscopy, Electron, Spiders, Amino Acids chemistry, Insect Proteins biosynthesis, Materials Testing, Silk metabolism

Abstract

Spider dragline silk is a remarkably strong fiber with impressive mechanical properties, which were thought to result from the specific structures of the underlying proteins and their molecular size. In this study, silk protein 11R26 from the dragline silk protein of Nephila clavipes was used to analyze the potential effects of the special amino acids on the function of 11R26. Three protein derivatives, ZF4, ZF5, and ZF6, were obtained by site-directed mutagenesis, based on the sequence of 11R26, and among these derivatives, serine was replaced with cysteine, isoleucine, and arginine, respectively. After these were expressed and purified, the mechanical performance of the fibers derived from the four proteins was tested. Both hardness and average elastic modulus of ZF4 fiber increased 2.2 times compared with those of 11R26. The number of disulfide bonds in ZF4 protein was 4.67 times that of 11R26, which implied that disulfide bonds outside the poly-Ala region affect the mechanical properties of spider silk more efficiently. The results indicated that the mechanical performances of spider silk proteins with small molecular size can be enhanced by modification of the amino acids residues. Our research not only has shown the feasibility of large-scale production of spider silk proteins but also provides valuable information for protein rational design.

Published

2016

115. Changes in 30K protein synthesis during delayed degeneration of the silk gland by a caspase-dependent pathway in a Bombyx (silkworm) mutant.

Author

Wang H, Wang Y, Wu C, Tao H, Chen X, Yin W, Sima Y, Wang Y, and Xu S

Subjects

Animals, Animals, Genetically Modified, Apoptosis, Bombyx genetics, Larva, Metamorphosis, Biological, Mutation, Protein Biosynthesis, Silk, Bombyx metabolism, Caspases metabolism, Insect Proteins biosynthesis

Abstract

The silk gland in silkworm (Bombyx mori) is a highly specialized organ that specifically synthesizes silk proteins. A function shift to the synthesis of large quantities of 30K proteins occurs in the degenerating silk gland cells during larval-pupal metamorphosis. The posterior silk gland developmental mutant model of silkworm was used in this study and changes in the programmed cell death (PCD) regulatory signals and 30K protein synthesis during silk gland degeneration were investigated. The results showed that PCD induced by 20-hydroxyecdysone was initiated early during larval-pupal metamorphosis in the mutant, but PCD proceeded slowly, resulting in the degeneration process of the silk gland being extended and took almost twice the time compared with the wild type. Caspase-dependent pathway signals regulated by Dronc in the silk gland cells of the mutant were significantly reduced, while the PCD initiation signal regulated by the Atg family was not delayed or reduced, and PCD-related epigenetic modification such as lysine methylation, acetylation, and succinylation, and tyrosine phosphorylation changed significantly. During the degeneration process in the mutant, 30K proteins were efficiently synthesized in the silk gland cells in stage PP1 even when no caspase protein was detected. Degeneration of the silk gland is a PCD process in which autophagy and apoptosis may participate. The degeneration process was regulated by a caspase-dependent pathway, while the synthesis of 30K proteins along with silk gland degeneration may not be entirely dependent on caspase signals.

Published

2016

116. Analysis of persistent changes to γ-aminobutyric acid receptor gene expression in Plutella xylostella subjected to sublethal amounts of spinosad.

Author

Yin XH, Wu QJ, Zhang YJ, Long YH, Wu XM, Li RY, Wang M, Tian XL, and Jiao XG

Subjects

Amino Acid Sequence, Animals, Drug Combinations, Gene Expression, Insect Proteins biosynthesis, Insect Proteins genetics, Insecticide Resistance, Moths metabolism, Receptors, GABA biosynthesis, Insecticides, Macrolides, Moths genetics, Receptors, GABA genetics

Abstract

A multi-generational approach was used to investigate the persistent effects of a sub-lethal dose of spinosad in Plutella xylostella. The susceptibility of various sub-populations of P. xylostella to spinosad and the effects of the insecticide on the gene expression of γ-aminobutyric acid receptor (GABAR) were determined. The results of a leaf dip bioassay showed that the sensitivity of P. xylostella to spinosad decreased across generations. The sub-strains had been previously selected based on a determined LC25 of spinosad. Considering that GABA-gated chloride channels are the primary targets of spinosad, the cDNA of P. xylostella was used to clone GABARα by using reverse transcription-polymerase chain reaction (RT-PCR). The mature peptide cDNA was 1477-bp long and contained a 1449-bp open reading frame encoding a protein of 483 amino acids. The resulting amino acid sequence was used to generate a neighbor-joining dendrogram, and homology search was conducted using NCBI BLAST. The protein had high similarity with the known GABAR sequence from P. xylostella. Subsequent semi-quantitative RT-PCR and real-time PCR analyses indicated that the GABAR transcript levels in the spinosad-resistant strain (RR, 145.82-fold) and in Sub1 strain (selected with LC25 spinosad for one generation) were the highest, followed by those in the spinosad-susceptible strain, the Sub10 strain (selected for ten generations), and the Sub5 strain (selected for five generations). This multi-generational study found significant correlations between spinosad susceptibility and GABAR gene expression, providing insights into the long-term effects of sub-lethal insecticide exposure and its potential to lead to the development of insecticide-resistant insect populations.

Published

2016

117. [REGULATION OF ANTIMICROBIAL PEPTIDE SYNTHESIS IN THE LARVAE OF CALLIPHORA VICINA (DIPTERA, CALLIPHORIDAE): DOSE-DEPENDENT EFFECT OF ECDYSTEROIDS].

Author

Gordya NA, Nesin AP, Simonenko NP, and Chernysh SI

Subjects

Animals, Antimicrobial Cationic Peptides immunology, Diptera immunology, Dose-Response Relationship, Drug, Ecdysterone immunology, Insect Proteins immunology, Larva metabolism, Antimicrobial Cationic Peptides biosynthesis, Diptera metabolism, Ecdysterone pharmacology, Insect Proteins biosynthesis

Abstract

Ecdysteroids are multifunctional hormones regulating virtually all morphogenetic processes in insects. Their role in stress and immune response regulation is less known. Here we studied 20-hydroxyecdysone effect on synthesis of the antimicrobial peptides in larvae of Calliphora vicina. An inverse correlation was found between 20-hydroxyecdysone titer and the concentration of antimicrobial peptides in the hemolymph of unaffected and bacteria-immunized insects. High and low doses of 20-hydroxyecdysone, injected simultaneously with bacterial cells, had an opposite effect on antimicrobial peptide synthesis in the diapausing larvae. Morphogenetically effective doses of 20-hydroxyecdysone demonstrated immuno-suppressive activity. Low doses of 20-hydroxyecdysone, on the contrary, moderately stimulated synthesis of the antimicrobial peptides. These data suggest that ecdysteroids are directly involved in regulation of the immune system activity and the final effect is dose-dependent.

Published

2016

118. Ecdysone signaling regulates soldier-specific cuticular pigmentation in the termite Zootermopsis nevadensis.

Author

Masuoka Y and Maekawa K

Subjects

Animals, Ecdysone genetics, Insect Proteins genetics, Isoptera genetics, Molting physiology, Receptors, Steroid genetics, Ecdysone metabolism, Gene Expression Regulation physiology, Insect Proteins biosynthesis, Isoptera metabolism, Pigmentation physiology, Receptors, Steroid biosynthesis

Abstract

Termite caste differentiation requires hormonal regulation, but understanding of the role of ecdysone is limited. Here, we investigated the expression and function of ecdysone-related genes during soldier differentiation in the damp-wood termite Zootermopsis nevadensis. Ecdysone receptor gene (EcR) was highly expressed in the head just after the presoldier molt. Knockdown of EcR expression in the early presoldier period inhibited the molts into soldiers. However, knockdown in the middle period affected tyrosine metabolic gene expression and inhibited soldier-specific cuticular tanning. These results suggest that ecdysone activation is involved in soldier-specific cuticle formation., (© 2016 Federation of European Biochemical Societies.)

Published

2016

119. The Gene Expression Program for the Formation of Wing Cuticle in Drosophila.

Author

Sobala LF and Adler PN

Subjects

Animals, Chitin metabolism, Drosophila growth & development, Drosophila ultrastructure, Gene Expression Regulation, Developmental, Insect Proteins genetics, Microscopy, Electron, Transmission, Pupa genetics, Pupa growth & development, Pupa ultrastructure, Wings, Animal growth & development, Wings, Animal metabolism, Wings, Animal ultrastructure, Zona Pellucida Glycoproteins genetics, Chitin genetics, Drosophila genetics, Insect Proteins biosynthesis, Zona Pellucida Glycoproteins biosynthesis

Abstract

The cuticular exoskeleton of insects and other arthropods is a remarkably versatile material with a complex multilayer structure. We made use of the ability to isolate cuticle synthesizing cells in relatively pure form by dissecting pupal wings and we used RNAseq to identify genes expressed during the formation of the adult wing cuticle. We observed dramatic changes in gene expression during cuticle deposition, and combined with transmission electron microscopy, we were able to identify candidate genes for the deposition of the different cuticular layers. Among genes of interest that dramatically change their expression during the cuticle deposition program are ones that encode cuticle proteins, ZP domain proteins, cuticle modifying proteins and transcription factors, as well as genes of unknown function. A striking finding is that mutations in a number of genes that are expressed almost exclusively during the deposition of the envelope (the thin outermost layer that is deposited first) result in gross defects in the procuticle (the thick chitinous layer that is deposited last). An attractive hypothesis to explain this is that the deposition of the different cuticle layers is not independent with the envelope instructing the formation of later layers. Alternatively, some of the genes expressed during the deposition of the envelope could form a platform that is essential for the deposition of all cuticle layers.

Published

2016

120. A Bemisia tabaci midgut protein interacts with begomoviruses and plays a role in virus transmission.

Author

Rana VS, Popli S, Saurav GK, Raina HS, Chaubey R, Ramamurthy VV, and Rajagopal R

Subjects

Animals, Begomovirus pathogenicity, Digestive System virology, Hemiptera metabolism, Hemiptera virology, Hemolymph metabolism, Hemolymph virology, India, Insect Proteins metabolism, Insect Vectors metabolism, Insect Vectors virology, Plant Diseases genetics, Virus Internalization, Begomovirus metabolism, Insect Proteins biosynthesis, Plant Diseases virology, Symbiosis genetics

Abstract

Begomoviruses are a major group of plant viruses, transmitted exclusively by Bemisia tabaci (Gennadius) in a persistent circulative non-propagative manner. The information regarding molecular and cellular basis underlying Begomovirus - whitefly interaction is very scarce. Evidences have suggested that the insect gut possesses some crucial protein receptors that allow specific entry of virus into the insect haemolymph. We have performed yeast two hybrid gut cDNA expression library screening against coat protein of Tomato leaf curl New Delhi virus (ToLCV) and Cotton leaf curl Rajasthan virus (CLCuV) as bait. Midgut protein (MGP) was the common protein found interacting with both ToLCV and CLCuV. MGP was localized in whole mount B. tabaci as well as in dissected guts through confocal microscopy. Pull down and dot blot assays confirmed in vitro interaction between ToLCV/CLCuV coat protein and MGP. Immunolocalization analysis also showed colocalization of ToLCV/CLCuV particles and MGP within insect's gut. Finally, anti-MGP antibody fed B. tabaci, exhibited 70% reduction in ToLCV transmission, suggesting a supportive role for MGP in virus transmission., (© 2015 John Wiley & Sons Ltd.)

Published

2016

121. Cuticular protein and transcription factor genes expressed during prepupal-pupal transition and by ecdysone pulse treatment in wing discs of Bombyx mori.

Author

Shahin R, Iwanaga M, and Kawasaki H

Subjects

Animals, Bombyx growth & development, Ecdysone genetics, Ecdysone metabolism, Gene Expression Regulation, Developmental, Insect Proteins genetics, Larva growth & development, Pupa growth & development, Transcription Factors biosynthesis, Transcription Factors genetics, Wings, Animal growth & development, Wings, Animal metabolism, Bombyx genetics, Insect Proteins biosynthesis, Larva genetics, Pupa genetics

Abstract

We aimed to understand the underlying mechanism that regulates successively expressed cuticular protein (CP) genes around pupation in Bombyx mori. Quantitative PCR was conducted to clarify the expression profile of CP genes and ecdysone-responsive transcription factor (ERTF) genes around pupation. Ecdysone pulse treatment was also conducted to compare the developmental profiles and the ecdysone induction of the CP and ERTF genes. Fifty-two CP genes (RR-1 13, RR-2 18, CPG 8, CPT 3, CPFL 2, CPH 8) in wing discs of B. mori were examined. Different expression profiles were found, which suggests the existence of a mechanism that regulates CP genes. We divided the genes into five groups according to their peak stages of expression. RR-2 genes were expressed until the day of pupation and RR-1 genes were expressed before and after pupation and for longer than RR-2 genes; this suggests different construction of exo- and endocuticular layers. CPG, CPT, CPFL and CPH genes were expressed before and after pupation, which implies their involvement in both cuticular layers. Expression profiles of ERTFs corresponded with previous reports. Ecdysone pulse treatment showed that the induction of CP and ERTF genes in vitro reflected developmental expression, from which we speculated that ERTFs regulate CP gene expression around pupation., (© 2016 The Royal Entomological Society.)

Published

2016

122. Dynamics and regulation of glycolysis-tricarboxylic acid metabolism in the midgut of Spodoptera litura during metamorphosis.

Author

Hu D, Luo W, Fan LF, Liu FL, Gu J, Deng HM, Zhang C, Huang LH, and Feng QL

Subjects

Animals, Digestive System metabolism, Gene Expression Regulation, Developmental, Insect Proteins biosynthesis, Insect Proteins genetics, Pupa genetics, Pupa growth & development, RNA, Messenger biosynthesis, Spodoptera growth & development, Starvation, Glycolysis genetics, Metamorphosis, Biological genetics, Spodoptera genetics, Tricarboxylic Acids metabolism

Abstract

Significant changes usually take place in the internal metabolism of insects during metamorphosis. The glycolysis-tricarboxylic acid (glycolysis-TCA) pathway is important for energy metabolism. To elucidate its dynamics, the mRNA levels of genes involved in this pathway were examined in the midgut of Spodoptera litura during metamorphosis, and the pyruvate content was quantified. The expression patterns of these genes in response to starvation were examined, and the interaction between protein phosphatase 1 (PP1) and phosphofructokinase (PFK) was studied. The results revealed that the expression or activities of most glycolytic enzymes was down-regulated in prepupae and then recovered in some degree in pupae, and all TCA-related genes were remarkably suppressed in both the prepupae and pupae. Pyruvate was enriched in the pupal midgut. Taken together, these results suggest that insects decrease both glycolysis and TCA in prepupae to save energy and then up-regulate glycolysis but down-regulate TCA in pupae to increase the supply of intermediates for construction of new organs. The expression of all these genes were down-regulated by starvation, indicating that non-feeding during metamorphosis may be a regulator of glycolysis-TCA pathway in the midgut. Importantly, interaction between PP1 and PFK was identified and is suggested to be involved in the regulation of glycolysis., (© 2015 The Royal Entomological Society.)

Published

2016

123. Evolution of Social Insect Polyphenism Facilitated by the Sex Differentiation Cascade.

Author

Klein A, Schultner E, Lowak H, Schrader L, Heinze J, Holman L, and Oettler J

Subjects

Animals, Ants physiology, DNA-Binding Proteins biosynthesis, DNA-Binding Proteins genetics, Drosophila Proteins biosynthesis, Drosophila Proteins genetics, Gene Expression Regulation, Developmental, Insect Proteins genetics, Kruppel-Like Transcription Factors biosynthesis, Kruppel-Like Transcription Factors genetics, Phenotype, Social Behavior, Ants genetics, Biological Evolution, Insect Proteins biosynthesis, Sex Differentiation genetics

Abstract

The major transition to eusociality required the evolution of a switch to canalize development into either a reproductive or a helper, the nature of which is currently unknown. Following predictions from the 'theory of facilitated variation', we identify sex differentiation pathways as promising candidates because of their pre-adaptation to regulating development of complex phenotypes. We show that conserved core genes, including the juvenile hormone-sensitive master sex differentiation gene doublesex (dsx) and a krüppel homolog 2 (kr-h2) with putative regulatory function, exhibit both sex and morph-specific expression across life stages in the ant Cardiocondyla obscurior. We hypothesize that genes in the sex differentiation cascade evolved perception of alternative input signals for caste differentiation (i.e. environmental or genetic cues), and that their inherent switch-like and epistatic behavior facilitated signal transfer to downstream targets, thus allowing them to control differential development into morphological castes.

Published

2016

124. Transcriptome and Expression Patterns of Chemosensory Genes in Antennae of the Parasitoid Wasp Chouioia cunea.

Author

Zhao Y, Wang F, Zhang X, Zhang S, Guo S, Zhu G, Liu Q, and Li M

Subjects

Animals, Female, Male, Smell physiology, Arthropod Antennae metabolism, Gene Expression Regulation physiology, Insect Proteins biosynthesis, Transcriptome physiology, Wasps metabolism

Abstract

Chouioia cunea Yang is an endoparasitic wasp that attacks pupae of Hyphantria cunea (Drury), an invasive moth species that severely damages forests in China. Chemosensory systems of insects are used to detect volatile chemical odors such as female sex pheromones and host plant volatiles. The antennae of parasite wasps are important for host detection and other sensory-mediated behaviors. We identified and documented differential expression profiles of chemoreception genes in C. cunea antennae. A total of 25 OBPs, 80 ORs, 10 IRs, 11 CSP, 1 SNMPs, and 17 GRs were annotated from adult male and female C. cunea antennal transcriptomes. The expression profiles of 25 OBPs, 16 ORs, and 17 GRs, 5 CSP, 5 IRs and 1 SNMP were determined by RT-PCR and RT-qPCR for the antenna, head, thorax, and abdomen of male and female C. cunea. A total of 8 OBPs, 14 ORs, and 8 GRs, 1 CSP, 4 IRs and 1 SNMPs were exclusively or primarily expressed in female antennae. These female antennal-specific or dominant expression profiles may assist in locating suitable host and oviposition sites. These genes will provide useful targets for advanced study of their biological functions.

Published

2016

125. Dusky-like is required for epidermal pigmentation and metamorphosis in Tribolium castaneum.

Author

Li C, Yun X, and Li B

Subjects

Animals, Epidermis metabolism, Fat Body metabolism, Female, Insect Proteins genetics, Membrane Proteins genetics, Organ Specificity, Ovary metabolism, Tribolium genetics, Gene Expression Regulation physiology, Insect Proteins biosynthesis, Membrane Proteins biosynthesis, Metamorphosis, Biological physiology, Pigmentation physiology, Tribolium metabolism

Abstract

Dusky-like (Dyl) is associated with the morphogenesis of embryonic denticle, adult sensory bristle and wing hair in Drosophila melanogaster. And whether Dyl involved in insect post-embryonic development and its signal transduction are poorly understood. Here, phylogenetic analysis revealed that dyl displayed one-to-one orthologous relationship among insects. In Tribolium castaneum, dyl is abundantly expressed at the late embryonic stage. Tissue-specific expression analysis at the late adult stage illustrated high expression of dyl in the fat body and ovary. Knockdown of dyl resulted in the defects in larval epidermal pigmentation and completely blocked the transitions from larval to pupal and pupal to adult stages of T. castaneum. We further discovered that dyl RNAi phenotypes were phenocopied by blimp-1 or shavenbaby (svb) silencing, and dyl was positively regulated by blimp-1 through svb in T. castaneum. These results suggest that Dyl functions downstream of Blimp-1 through Svb for larval epidermal pigmentation and metamorphosis. Moreover, ftz-f1 was down-regulated after RNA interference (RNAi) suppressing any of those three genes, indicating that Ftz-f1 works downstream of Dyl to mediate the effects of Blimp-1, Svb and Dyl on metamorphosis in T. castaneum. This study provides valuable insights into functions and signaling pathway of insect Dyl.

Published

2016

126. Identification of heat shock cognate protein 70 gene (Alhsc70) of Apolygus lucorum and its expression in response to different temperature and pesticide stresses.

Author

Sun Y, Zhao J, Sheng Y, Xiao YF, Zhang YJ, Bai LX, Tan Y, Xiao LB, and Xu GC

Subjects

Amino Acid Sequence, Animals, Base Sequence, Cloning, Molecular, Gene Expression Regulation drug effects, HSP70 Heat-Shock Proteins biosynthesis, HSP70 Heat-Shock Proteins chemistry, HSP70 Heat-Shock Proteins metabolism, Heteroptera drug effects, Heteroptera physiology, Insect Proteins biosynthesis, Insect Proteins chemistry, Insect Proteins metabolism, Molecular Sequence Data, Phylogeny, Transcription, Genetic drug effects, HSP70 Heat-Shock Proteins genetics, Heteroptera genetics, Insect Proteins genetics, Pesticides pharmacology, Stress, Physiological drug effects, Stress, Physiological genetics, Temperature

Abstract

Heat shock cognate protein 70 (Hsc70) is a very important stress-resistance protein of insects against environmental stresses. We employed fluorescent real-time quantitative polymerase chain reaction and Western-blot techniques to analyze the transcriptional and translational expression profiles of AlHSC70 under extreme temperature (4°C and 40°C) or 4 pesticide stresses in Apolygus lucorum. The results showed that the expression of AlHSC70 were significantly induced by cyhalothrin or extremely high temperature (40°C) in both transcriptional and translational levels (P < 0.05), while the transcriptional and translational level of AlHSC70 decreased significantly in treatments of chlorpyrifos or extreme cold temperature (4°C) (P < 0.05). Moreover, after Apolygus lucorum treated by imidacloprid or emamectin benzoate, the expression of AlHSC70 was only up-regulated significantly at the transcriptional level (P < 0.05), although obviously up-regulated at the translational level of AlHSC70. Therefore, this study confirmed that the Alhsc70 gene played important roles in response to both temperature and pesticide stresses, especially for cyhalothrin or extremely high temperature (40°C). In addition, the significant polynomial regression correlations between temperature and the Alhsc70 expression level were shown in all the nymph and adult stages (P < 0.01), indicating temperature was an important factor to affect the relative expression of Alhsc70., (© 2014 Institute of Zoology, Chinese Academy of Sciences.)

Published

2016

127. Antibacterial Peptide CecropinB2 Production via Various Host and Construct Systems.

Author

Lai WS, Kan SC, Lin CC, Shieh CJ, and Liu YC

Subjects

Acinetobacter baumannii drug effects, Acinetobacter baumannii growth & development, Antimicrobial Cationic Peptides biosynthesis, Antimicrobial Cationic Peptides pharmacology, Bacillus subtilis drug effects, Bacillus subtilis growth & development, Bacillus subtilis metabolism, Escherichia coli drug effects, Escherichia coli growth & development, Escherichia coli metabolism, Gene Expression, Genetic Vectors chemistry, Genetic Vectors metabolism, Insect Proteins biosynthesis, Insect Proteins pharmacology, Inteins genetics, Microbial Sensitivity Tests, Pichia metabolism, Plasmids chemistry, Plasmids metabolism, Protein Engineering, Protein Sorting Signals, Recombinant Fusion Proteins biosynthesis, Recombinant Fusion Proteins pharmacology, Antimicrobial Cationic Peptides genetics, Bacillus subtilis genetics, Escherichia coli genetics, Insect Proteins genetics, Pichia genetics, Recombinant Fusion Proteins genetics

Abstract

Cecropin is a cationic antibacterial peptide composed of 35-39 residues. This peptide has been identified as possessing strong antibacterial activity and low toxicity against eukaryotic cells, and it has been claimed that some types of the cecropin family of peptides are capable of killing cancer cells. In this study, the host effect of cloning antibacterial peptide cecropinB2 was investigated. Three different host expression systems were chosen, i.e., Escherichia coli, Bacillus subtilis and Pichia pastoris. Two gene constructs, cecropinB2 (cecB2) and intein-cecropinB2 (INT-cecB2), were applied. Signal peptide and propeptide from Armigeres subalbatus were also attached to the gene construct. The results showed that the best host for cloning cecropinB2 was P. pastoris SMD1168 harboring the gene of pGAPzαC-prepro-cecB2 via Western blot confirmation. The cecropinB2 that was purified using immobilized-metal affinity chromatography resin showed strong antibacterial activity against the Gram-negative strains, including the multi-drug-resistant bacteria Acinetobacter baumannii.

Published

2016

128. Molecular cloning, expression, purification and characterization of a novel cellulase gene (Bh-EGaseI) in the beetle Batocera horsfieldi.

Author

Mei HZ, Xia DG, Zhao QL, Zhang GZ, Qiu ZY, Qian P, and Lu C

Subjects

Animals, Cloning, Molecular, Gene Expression, Recombinant Proteins biosynthesis, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins isolation & purification, Cellulase biosynthesis, Cellulase chemistry, Cellulase genetics, Cellulase isolation & purification, Coleoptera enzymology, Coleoptera genetics, Insect Proteins biosynthesis, Insect Proteins chemistry, Insect Proteins genetics, Insect Proteins isolation & purification

Abstract

Wood-feeding insects depend heavily on the secretion of a combination of cellulases, mainly endoglucanases and other glucanases such as exoglucanases and xylanases, to achieve efficient digestion of the cellulose of cellulosic materials. In this paper, we report a novel cellulose Bh-EGaseI belonging to the glycoside hydrolase family 45(gh45-1) obtained from the beetle Batocera horsfieldi. The Bh-EGaseI gene spans 714 bp and consists of three exons coding 237 amino acid residues. The cDNA encoding Bh-EGaseI was expressed as 25 KDa in baculovirus-infected Bombyx mori larvae. The expression products of Bh-EGaseI from larval hemolymph showed a specific enzymatic activity of approximately 1030.87 IU per mg. The enzyme was active over a wide range of pH and temperatures; optimal activity was observed at 40 °C and pH 4.0. The effects of ions on Bh-EGaseI activity were also studied, and results indicated that activity decreased to different extents upon addition of ions. Investigations on Bh-EGaseI facilitate their potential application in the production of bioenergy and biomaterials from cellulosic biomass in the future., (Copyright © 2015 Elsevier B.V. All rights reserved.)

Published

2016

129. Cloning and analysis of DnaJ family members in the silkworm, Bombyx mori.

Author

Li Y, Bu C, Li T, Wang S, Jiang F, Yi Y, Yang H, and Zhang Z

Subjects

Animals, Cloning, Molecular, Databases, Genetic, Hemocytes metabolism, Organ Specificity physiology, Protein Structure, Tertiary, Bombyx genetics, Bombyx metabolism, Gene Expression Regulation physiology, HSP40 Heat-Shock Proteins biosynthesis, HSP40 Heat-Shock Proteins genetics, Insect Proteins biosynthesis, Insect Proteins genetics, Phylogeny

Abstract

Heat shock proteins (Hsps) are involved in a variety of critical biological functions, including protein folding, degradation, and translocation and macromolecule assembly, act as molecular chaperones during periods of stress by binding to other proteins. Using expressed sequence tag (EST) and silkworm (Bombyx mori) transcriptome databases, we identified 27 cDNA sequences encoding the conserved J domain, which is found in DnaJ-type Hsps. Of the 27 J domain-containing sequences, 25 were complete cDNA sequences. We divided them into three types according to the number and presence of conserved domains. By analyzing the gene structures, intron numbers, and conserved domains and constructing a phylogenetic tree, we found that the DnaJ family had undergone convergent evolution, obtaining new domains to expand the diversity of its family members. The acquisition of the new DnaJ domains most likely occurred prior to the evolutionary divergence of prokaryotes and eukaryotes. The expression of DnaJ genes in the silkworm was generally higher in the fat body. The tissue distribution of DnaJ1 proteins was detected by western blotting, demonstrating that in the fifth-instar larvae, the DnaJ1 proteins were expressed at their highest levels in hemocytes, followed by the fat body and head. We also found that the DnaJ1 transcripts were likely differentially translated in different tissues. Using immunofluorescence cytochemistry, we revealed that in the blood cells, DnaJ1 was mainly localized in the cytoplasm., (Copyright © 2015 Elsevier B.V. All rights reserved.)

Published

2016

130. Expression signature of some immunity genes triggered in Apis mellifera carpatica model by Pseudomonas entomophila experimental infection.

Author

Neagu A, Raþiu AC, Mihalache (Radu) MR, Lazãr V, Chifiriuc MC, and Ecovoiu AA

Subjects

Animal Diseases microbiology, Animals, Bees immunology, Bees microbiology, Drosophila melanogaster genetics, Drosophila melanogaster immunology, Insect Proteins genetics, Insect Proteins immunology, Real-Time Polymerase Chain Reaction, Species Specificity, Bees genetics, Gene Expression Profiling, Genes, Insect, Immunity, Innate genetics, Insect Proteins biosynthesis, Pseudomonas pathogenicity

Abstract

Herein we report the expression profiles of certain immunity genes from Apis mellifera carpatica worker individuals experimentally infected with Pseudomonas entomophila L48 strain. Changes of the relative expression of abaecin, Relish, dorsal, Toll-1, domeless, and Duox genes were monitored by qRT-PCR. Our results were compared with similar ones from Drosophila melanogaster model and suggest that these genes are involved in the anti-infective defense mechanisms. Our study opens investigation avenues for modern prophylactic and therapeutic approaches of infections affecting the honeybees, but also for identifying new orthologous genes involved in the human innate immune response.

Published

2016

131. Immune response and survival of Circulifer haematoceps to Spiroplasma citri infection requires expression of the gene hexamerin.

Author

Eliautout R, Dubrana MP, Vincent-Monégat C, Vallier A, Braquart-Varnier C, Poirié M, Saillard C, Heddi A, and Arricau-Bouvery N

Subjects

Animals, Gene Knockdown Techniques, Hemiptera genetics, Insect Proteins immunology, Insect Vectors microbiology, Polymerase Chain Reaction, Spiroplasma citri immunology, Gram-Negative Bacterial Infections immunology, Hemiptera immunology, Hemiptera microbiology, Insect Proteins biosynthesis, Insect Vectors immunology

Abstract

Spiroplasma citri is a cell wall-less bacterium that infects plants. It is transmitted by the leafhopper Circulifer haematoceps, which hosts this bacterium in the haemocel and insect tissues. Bacterial factors involved in spiroplasma colonization of the insect host have been identified, but the immune response of the leafhopper to S. citri infection remains unknown. In this study, we showed that C. haematoceps activates both humoral and cellular immune responses when challenged with bacteria. When infected by S. citri, C. haematoceps displayed a specific immune response, evidenced by activation of phagocytosis and upregulation of a gene encoding the protein hexamerin. S. citri infection also resulted in decreased phenoloxidase-like activity. Inhibition of hexamerin by RNA interference resulted in a significant reduction in phenoloxidase-like activity and increased mortality of infected leafhoppers. Therefore, the gene hexamerin is involved in S. citri control by interfering with insect phenoloxidase activity., (Copyright © 2015 Elsevier Ltd. All rights reserved.)

Published

2016

132. The effects of Bombyx mori silk strain and extraction time on the molecular and biological characteristics of sericin.

Author

Siritientong T, Bonani W, Motta A, Migliaresi C, and Aramwit P

Subjects

Animals, Bombyx metabolism, Cell Proliferation drug effects, Chromatography, Reverse-Phase, Gene Expression, Insect Proteins biosynthesis, Insect Proteins isolation & purification, Insect Proteins pharmacology, Liquid-Liquid Extraction methods, Mice, Molecular Weight, NIH 3T3 Cells, Sericins biosynthesis, Sericins isolation & purification, Sericins pharmacology, Time Factors, Amino Acids chemistry, Bombyx genetics, Insect Proteins chemistry, Sericins chemistry

Abstract

Sericin was extracted from three strains of Thai Bombyx mori silk cocoons (white shell Chul1/1, greenish shell Chul3/2, and yellow shell Chul4/2) by a high-pressure and high-temperature technique. The characteristics of sericin extracted from different fractions (15, 45, and 60 min extraction process) were compared. No differences in amino acid composition were observed among the three fractions. For all silk strains, sericin extracted from a 15-min process presented the highest molecular weight. The biological potential of the different sericin samples as a bioadditive for 3T3 fibroblast cells was assessed. When comparing sericin extracted from three silk strains, sericin fractions extracted from Chul4/2 improved cell proliferation, while sericin from Chul 1/1 activated Type I collagen production to the highest extent. This study allows the natural variability of sericin obtained from different sources and extraction conditions to be addressed and provides clues for the selection of sericin sources.

Published

2016

133. Plasmodium falciparum suppresses the host immune response by inducing the synthesis of insulin-like peptides (ILPs) in the mosquito Anopheles stephensi.

Author

Pietri JE, Pietri EJ, Potts R, Riehle MA, and Luckhart S

Subjects

Animals, Extracellular Signal-Regulated MAP Kinases metabolism, Insect Proteins biosynthesis, Insect Proteins genetics, Insulin analogs & derivatives, Intercellular Signaling Peptides and Proteins genetics, MAP Kinase Signaling System immunology, Malaria, Falciparum immunology, Malaria, Falciparum parasitology, Mitogen-Activated Protein Kinase Kinases metabolism, Phosphatidylinositol 3-Kinase metabolism, Proto-Oncogene Proteins c-akt metabolism, Somatomedins metabolism, Anopheles immunology, Anopheles parasitology, Insect Hormones genetics, Peptide Hormones genetics, Plasmodium falciparum immunology

Abstract

The insulin-like peptides (ILPs) and their respective signaling and regulatory pathways are highly conserved across phyla. In invertebrates, ILPs regulate diverse physiological processes, including metabolism, reproduction, behavior, and immunity. We previously reported that blood feeding alone induced minimal changes in ILP expression in Anopheles stephensi. However, ingestion of a blood meal containing human insulin or Plasmodium falciparum, which can mimic insulin signaling, leads to significant increases in ILP expression in the head and midgut, suggesting a potential role for AsILPs in the regulation of P. falciparum sporogonic development. Here, we show that soluble P. falciparum products, but not LPS or zymosan, directly induced AsILP expression in immortalized A. stephensi cells in vitro. Further, AsILP expression is dependent on signaling by the mitogen-activated protein kinase kinase/extracellular signal-regulated kinase (MEK/ERK) and phosphatidylinositol 3'-kinase (PI3K)/Akt branches of the insulin/insulin-like growth factor signaling (IIS) pathway. Inhibition of P. falciparum-induced ILPs in vivo decreased parasite development through kinetically distinct effects on mosquito innate immune responses. Specifically, knockdown of AsILP4 induced early expression of immune effector genes (1-6 h after infection), a pattern associated with significantly reduced parasite abundance prior to invasion of the midgut epithelium. In contrast, knockdown of AsILP3 increased later expression of the same genes (24 h after infection), a pattern that was associated with significantly reduced oocyst development. These data suggest that P. falciparum parasites alter the expression of mosquito AsILPs to dampen the immune response and facilitate their development in the mosquito vector., (Copyright © 2015 Elsevier Ltd. All rights reserved.)

Published

2015

134. A novel Lozenge gene in silkworm, Bombyx mori regulates the melanization response of hemolymph.

Author

Xu M, Wang X, Tan J, Zhang K, Guan X, Patterson LH, Ding H, and Cui H

Subjects

Animals, Cell Differentiation immunology, Core Binding Factor alpha Subunits genetics, Gene Expression Profiling, Hemocytes cytology, Hemocytes metabolism, Immunity, Innate immunology, Insect Proteins biosynthesis, Insect Proteins genetics, Insect Proteins immunology, RNA Interference, RNA, Small Interfering, Transcription Factors biosynthesis, Transcription Factors genetics, Transcription Factors immunology, Bombyx genetics, Bombyx immunology, Catechol Oxidase biosynthesis, Enzyme Precursors biosynthesis, Hemolymph immunology, Melanins metabolism

Abstract

Runt-related (RUNX) transcription factors are evolutionarily conserved either in vertebrate or invertebrate. Lozenge (Lz), a members of RUNX family as well as homologue of AML-1, functions as an important transcription factor regulating the hemocytes differentiation. In this paper, we identified and characterized RUNX family especially Lz in silkworm, which is a lepidopteran model insect. The gene expression analysis illustrated that BmLz was highly expressed in hemocytes throughout the whole development period, and reached a peak in glutonous stage. Over-expression of BmLz in silkworm accelerated the melanization process of hemolymph, and led to instantaneously up-regulation of prophenoloxidases (PPOs), which were key enzymes in the melanization process. Further down-regulation of BmLz expression by RNA interference resulted in the significant delay of melanization reaction of hemolymph. These findings suggested that BmLz regulated the melanization process of hemolymph by inducing PPOs expression, and played a critical role in innate immunity defense in silkworm., (Copyright © 2015 Elsevier Ltd. All rights reserved.)

Published

2015

135. Weevil endosymbiont dynamics is associated with a clamping of immunity.

Author

Masson F, Moné Y, Vigneron A, Vallier A, Parisot N, Vincent-Monégat C, Balmand S, Carpentier MC, Zaidman-Rémy A, and Heddi A

Subjects

Animals, Apoptosis genetics, Autophagy genetics, Bacteria genetics, Base Sequence, Digestive System microbiology, High-Throughput Nucleotide Sequencing, Insect Proteins biosynthesis, Larva growth & development, Larva immunology, Larva microbiology, Weevils growth & development, Weevils microbiology, Insect Proteins genetics, Symbiosis genetics, Weevils genetics, Weevils immunology

Abstract

Background: Insects subsisting on nutritionally unbalanced diets have evolved long-term mutualistic relationships with intracellular symbiotic bacteria (endosymbionts). The endosymbiont population load undergoes changes along with insect development. In the cereal weevil Sitophilus oryzae, the midgut endosymbionts Sodalis pierantonius drastically multiply following adult metamorphosis and rapidly decline until total elimination when the insect achieves its cuticle synthesis. Whilst symbiont load was shown to timely meet insect metabolic needs, little is known about the host molecular and immune processes underlying this dynamics., Methods: We performed RNA sequencing analysis on weevil midguts at three representative phases of the endosymbiont dynamics (i.e. increase, climax and decrease). To screen genes which transcriptional changes are specifically related to symbiont dynamics and not to the intrinsic development of the midgut, we further have monitored by RT-qPCR sixteen gene transcript levels in symbiotic and artificially non-symbiotic (aposymbiotic) weevils. We also localized the endosymbionts during the elimination process by fluorescence microscopy., Results: Functional analysis of the host differentially expressed genes by RNA sequencing showed that the main transcriptional changes occur during endosymbiont growth phase and affect cell proliferation, apoptosis, autophagy, phagocytosis, and metabolism of fatty acids and nucleic acids. We also showed that symbiont dynamics alters the expression of several genes involved in insect development. Our results strengthened the implication of apoptosis and autophagy processes in symbiont elimination and recycling. Remarkably, apart from the coleoptericin A that is known to target endosymbionts and controls their division and location, no gene coding antimicrobial peptide was upregulated during the symbiont growth and elimination phases., Conclusion: We show that endosymbiont dynamics parallels numerous transcriptional changes in weevil developing adults and affects several biological processes, including metabolism and development. It also triggers cell apoptosis, autophagy and gut epithelial cell swelling and delamination. Strikingly, immunity is repressed during the whole process, presumably avoiding tissue inflammation and allowing insects to optimize nutrient recovery from recycled endosymbiont.

Published

2015

136. High yield exogenous protein HPL production in the Bombyx mori silk gland provides novel insight into recombinant expression systems.

Author

Wang H, Wang L, Wang Y, Tao H, Yin W, SiMa Y, Wang Y, and Xu S

Subjects

Animals, Animals, Genetically Modified, Computational Biology methods, Gene Expression Profiling, Gene Expression Regulation, Genetic Vectors genetics, Mutation, Phenotype, Bombyx genetics, Bombyx metabolism, Gene Expression, Insect Proteins biosynthesis, Insect Proteins genetics, Recombinant Proteins, Silk biosynthesis

Abstract

The silk gland of Bombyx mori (BmSG) has gained significant attention by dint of superior synthesis and secretion of proteins. However, the application of BmSG bioreactor is still a controversial issue because of low yields of recombinant proteins. Here, a 3057 bp full-length coding sequence of Hpl was designed and transformed into the silkworm genome, and then the mutant (Hpl/Hpl) with specific expression of Hpl in posterior BmSG (BmPSG) was obtained. In the mutants, the transcription level of Fib-L and P25, and corresponding encoding proteins, did not decrease. However, the mRNA level of Fib-H was reduced by 71.1%, and Fib-H protein in the secreted fibroin was decreased from 91.86% to 71.01%. The mRNA level of Hpl was 0.73% and 0.74% of Fib-H and Fib-L, respectively, while HPL protein accounted for 18.85% of fibroin and 15.46% of the total amount of secreted silk protein. The exogenous protein was therefore very efficiently translated and secreted. Further analysis of differentially expressed gene (DEG) was carried out in the BmPSG cells and 891 DEGs were detected, of which 208 genes were related to protein metabolism. Reduced expression of endogenous silk proteins in the BmPSG could effectively improve the production efficiency of recombinant exogenous proteins.

Published

2015

137. Instar-dependent systemic RNA interference response in Leptinotarsa decemlineata larvae.

Author

Guo WC, Fu KY, Yang S, Li XX, and Li GQ

Subjects

Adenosylhomocysteinase biosynthesis, Animals, Argonaute Proteins biosynthesis, Coleoptera genetics, Insect Proteins biosynthesis, Larva, Ribonuclease III biosynthesis, Coleoptera metabolism, RNA Interference

Abstract

RNA interference (RNAi) is a promising approach to control Leptinotarsa decemlineata. In this study, RNAi efficiency by double-stranded RNA (dsRNA) targeting S-adenosyl-L-homocysteine hydrolase (LdSAHase) was compared among L. decemlineata first- to fourth-instar larvae. Ingesting dsLdSAHase successfully decreased the target gene expression, caused lethality, inhibited growth and impaired pupation in an instar- and concentration-dependent manner. To study the role of Dicer2 and Argonaute2 genes in RNAi efficiency, we identified LdDcr2a, LdDcr2b, LdAgo2a and LdAgo2b. Their expression levels were higher in young larvae than those in old ones. Exposure to dsegfp for 6 h significantly elevated LdDcr2a, LdDcr2b, LdAgo2a and LdAgo2b mRNA levels in the first-, second-, third- and fourth-instar larvae. When the exposure periods were extended, however, the expression levels were gradually reduced. Continuous exposure for 72 h significantly repressed the expression of LdAgo2a and LdAgo2b in the first, second and third larval instars, and the four genes in final instars. Moreover, we found that dsLdSAHase-caused LdSAHase suppressions and larval mortalities were influenced by previous dsegfp exposure: 12 h of previous exposure increased LdSAHase silencing and mortality of the final instar larvae, whereas 72 h of exposure reduced LdSAHase silencing and mortality. Thus, it seems the activities of core RNAi-machinery proteins affect RNAi efficiency in L. decemlineata., (Copyright © 2015 Elsevier Inc. All rights reserved.)

Published

2015

138. Transcriptome Analysis of Thermal Parthenogenesis of the Domesticated Silkworm.

Author

Liu P, Wang Y, Du X, Yao L, Li F, and Meng Z

Subjects

Animals, Female, Bombyx metabolism, Gene Expression Regulation, Hot Temperature, Insect Proteins biosynthesis, Parthenogenesis, Transcriptome

Abstract

Thermal induction of parthenogenesis (also known as thermal parthenogenesis) in silkworms is an important technique that has been used in artificial insemination, expansion of hybridization, transgenesis and sericultural production; however, the exact mechanisms of this induction remain unclear. This study aimed to investigate the gene expression profile in silkworms undergoing thermal parthenogenesis using RNA-seq analysis. The transcriptome profiles indicated that in non-induced and induced eggs, the numbers of differentially expressed genes (DEGs) for the parthenogenetic line (PL) and amphigenetic line (AL) were 538 and 545, respectively, as determined by fold-change ≥ 2. Gene ontology (GO) analysis showed that DEGs between two lines were mainly involved in reproduction, formation of chorion, female gamete generation and cell development pathways. Upregulation of many chorion genes in AL suggests that the maturation rate of AL eggs was slower than PL eggs. Some DEGs related to reactive oxygen species removal, DNA repair and heat shock response were differentially expressed between the two lines, such as MPV-17, REV1 and HSP68. These results supported the view that a large fraction of genes are differentially expressed between PL and AL, which offers a new approach to identifying the molecular mechanism of silkworm thermal parthenogenesis.

Published

2015

139. Proteomic changes occurring in the malaria mosquitoes Anopheles gambiae and Anopheles stephensi during aging.

Author

Sikulu MT, Monkman J, Dave KA, Hastie ML, Dale PE, Kitching RL, Killeen GF, Kay BH, Gorman JJ, and Hugo LE

Subjects

Animals, Anopheles parasitology, Malaria transmission, Plasmodium, Aging physiology, Anopheles metabolism, Gene Expression Regulation physiology, Insect Proteins biosynthesis, Proteomics

Abstract

The age of mosquitoes is a crucial determinant of their ability to transmit pathogens and their resistance to insecticides. We investigated changes to the abundance of proteins found in heads and thoraces of the malaria mosquitoes Anopheles gambiae and Anopheles stephensi as they aged. Protein expression changes were assessed using two-dimensional difference gel electrophoresis and the identity of differentially expressed proteins was determined by using either matrix-assisted laser desorption ionization tandem time-of-flight mass spectrometry or capillary high-pressure liquid chromatography coupled with a linear ion-trap (LTQ)-Orbitrap XL hybrid mass spectrometer. Protein biomarkers were validated by semi quantitative Western blot analysis. Nineteen and nine age dependent protein spots were identified for A. stephensi and A. gambiae, respectively. Among the proteins down-regulated with age were homologs of ADF/Cofilin, cytochome c1, heat shock protein-70 and eukaryotic translation initiation factor 5A (eIF5a). Proteins up-regulated with age included probable methylmalonate-semialdehyde dehydrogenase, voltage-dependent anion-selective channel and fructose bisphosphate aldolase. Semi quantitative Western blot analysis confirmed expression patterns observed by 2-D DIGE for eIF5a and ADF/Cofilin. Further work is recommended to determine whether these biomarkers are robust to infection, blood feeding and insecticide resistance. Robust biomarkers could then be incorporated into rapid diagnostic assays for ecological and epidemiological studies., Biological Significance: In this study, we have identified several proteins with characteristic changes in abundance in both A. gambiae and A. stephensi during their aging process. These changes may highlight underlying mechanisms beneath the relationship between mosquito age and factors affecting Plasmodium transmission and mosquito control. The similarity of changes in protein abundance between these species and the primary dengue vector Aedes aegypti, has revealed conserved patterns of aging-specific protein regulation., (Copyright © 2015 Elsevier B.V. All rights reserved.)

Published

2015

140. Impacts on silkworm larvae midgut proteomics by transgenic Trichoderma strain and analysis of glutathione S-transferase sigma 2 gene essential for anti-stress response of silkworm larvae.

Author

Li Y, Dou K, Gao S, Sun J, Wang M, Fu K, Yu C, Wu Q, Li Y, and Chen J

Subjects

Animals, Larva enzymology, Larva microbiology, Trichoderma genetics, Bombyx enzymology, Bombyx microbiology, Gene Expression Regulation, Enzymologic, Glutathione Transferase biosynthesis, Insect Proteins biosynthesis, Intestines enzymology, Intestines microbiology, Trichoderma growth & development

Abstract

Lepidoptera is a large order of insects that have major impacts on humans as agriculture pests. The midgut is considered an important target for insect control. In the present study, 10 up-regulated, 18 down-regulated, and one newly emerged protein were identified in the transgenic Trichoderma-treated midgut proteome. Proteins related to stress response, biosynthetic process, and metabolism process were further characterized through quantitative real-time PCR (qPCR). Of all the identified proteins, the glutathione S-transferase sigma 2 (GSTs2) gene displayed enhanced expression when larvae were fed with Trichoderma wild-type or transgenic strains. Down regulation of GSTs2 expression by RNA interference (RNAi) resulted in inhibition of silkworm growth when larvae were fed with mulberry leaves treated with the transgenic Trichoderma strain. Weight per larva decreased by 18.2%, 11.9%, and 10.7% in the untreated control, ddH2O, and GFP dsRNA groups, respectively, at 24h, while the weight decrease was higher at 42.4%, 28.8% and 32.4% at 72 h after treatment. Expression of glutathione S-transferase omega 2 (GSTo2) was also enhanced when larvae were fed with mulberry leaves treated with the transgenic Trichoderma strain. These results indicated that there was indeed correlation between enhanced expression of GSTs2 and the anti-stress response of silkworm larvae against Trichoderma. This study represents the first attempt at understanding the effects of transgenic organisms on the midgut proteomic changes in silkworm larvae. Our findings could not only broaden the biological control targets of insect at the molecular level, but also provide a theoretical foundation for biological safety evaluation of the transgenic Trichoderma strain., (Copyright © 2015 Elsevier B.V. All rights reserved.)

Published

2015

141. [Yeast expression and application of an antifreeze protein from the desert beetle Microdera punctipennis].

Author

Meng S, Cai W, and Ma J

Subjects

Animals, Blotting, Western, Cold Temperature, Electrophoresis, Polyacrylamide Gel, Freezing, Mice, Pichia metabolism, Sf9 Cells, Antifreeze Proteins biosynthesis, Coleoptera, Cryoprotective Agents chemistry, Insect Proteins biosynthesis

Abstract

Insect antifreeze protein (AFP) has high antifreeze activity. Antifreeze proteins can be used in cryopreservation of biological tissues and cells. We expressed an antifreeze protein from the desert beetle Microdera punctipennis in yeast and determined the function of the protein at low temperatures. Yeast expression vector, pPIC9K-Mpafp698, was constructed and transformed into Pichia pastoris GS115. The expression of MpAFP698 was induced by methanol, and identified by tricine SDS-PAGE and Western blotting. Mpafp698 gene was inserted into the genome of the host yeast strain GS115, and correctly expressed. Hardly any yeast's own protein was secreted into the media. Cryoprotective experiments showed that MpAFP698 can significantly protect mouse liver as well as other mouse organs from cold damage compared with those in the control of Bovine serum albumin (BSA) addition. Besides, the hemolysis of blood cells protected by MpAFP698 at 4 degrees C was reduced and the survival rate of SF9 cells protected by MpAFP698 after freezing and thawing was increased compared to those of the control with BSA addition. Our results showed that MpAFP698 can be expressed in yeast, which allows a convenient purification of the MpAFP protein that has the cryoprotective effect.

Published

2015

142. Mass Production of an Active Peptide-N-Glycosidase F Using Silkworm-Baculovirus Expression System.

Author

Masuda A, Xu J, Mitsudome T, Nagata Y, Morokuma D, Mon H, Banno Y, Kusakabe T, and Lee JM

Subjects

Animals, Cell Line, Insect Proteins genetics, Peptide-N4-(N-acetyl-beta-glucosaminyl) Asparagine Amidase genetics, Recombinant Proteins biosynthesis, Recombinant Proteins genetics, Baculoviridae, Bombyx, Gene Expression, Insect Proteins biosynthesis, Peptide-N4-(N-acetyl-beta-glucosaminyl) Asparagine Amidase biosynthesis

Abstract

The peptide-N (4)-(N-acetyl-β-D-glucosaminyl) asparagine amidase F (PNGase F) catalyzes the cleavage of N-linked oligosaccharides between the innermost GlcNAc and asparagine residues of high mannose, hybrid and complex oligosaccharides from glycoproteins. The PNGase F has broad substrate specificity and thus is extensively used for the structural and functional studies of the glycoproteins. In this study, we tried to produce active recombinant PNGase F as secreted and intracellular-expressed forms using baculovirus expression vector system (BEVS) through silkworm larvae or cultured cells. PNGase F itself contains potential N-linked glycosylation sites and we found that it was N-glycosylated when PNGase F secreted from silkworm cells. Intriguingly, the secreted recombinant PNGase F has the lower catalytic activity and self-digests its N-linked glycans and therefore this secreted form of this enzyme produced from BEVS is not appropriate for carbohydrate chain analysis. Instead, we successfully mass-produced (2.1 mg/20 silkworm larvae) and purified active recombinant PNGase F as an intracellular protein without N-glycosylations. Besides, we confirmed by directed mutagenesis that several amino acid residues are crucial for the function of PNGase F. Our results provide an alternative method for the mass production of active enzymes involved in the study of glycoproteins.

Published

2015

143. Increased Acetylcholinesterase Expression in Bumble Bees During Neonicotinoid-Coated Corn Sowing.

Author

Samson-Robert O, Labrie G, Mercier PL, Chagnon M, Derome N, and Fournier V

Subjects

Animals, Acetylcholinesterase biosynthesis, Anabasine pharmacology, Bees enzymology, Gene Expression Regulation, Enzymologic drug effects, Insect Proteins biosynthesis, Seeds, Zea mays

Abstract

While honey bee exposure to systemic insecticides has received much attention, impacts on wild pollinators have not been as widely studied. Neonicotinoids have been shown to increase acetylcholinesterase (AChE) activity in honey bees at sublethal doses. High AChE levels may therefore act as a biomarker of exposure to neonicotinoids. This two-year study focused on establishing whether bumble bees living and foraging in agricultural areas using neonicotinoid crop protection show early biochemical signs of intoxication. Bumble bee colonies (Bombus impatiens) were placed in two different agricultural cropping areas: 1) control (≥ 3 km from fields planted with neonicotinoid-treated seeds) or 2) exposed (within 500 m of fields planted with neonicotinoid-treated seeds), and maintained for the duration of corn sowing. As determined by Real Time qPCR, AChE mRNA expression was initially significantly higher in bumble bees from exposed sites, then decreased throughout the planting season to reach a similar endpoint to that of bumble bees from control sites. These findings suggest that exposure to neonicotinoid seed coating particles during the planting season can alter bumble bee neuronal activity. To our knowledge, this is the first study to report in situ that bumble bees living in agricultural areas exhibit signs of neonicotinoid intoxication.

Published

2015

144. Primed Immune Responses Triggered by Ingested Bacteria Lead to Systemic Infection Tolerance in Silkworms.

Author

Miyashita A, Takahashi S, Ishii K, Sekimizu K, and Kaito C

Subjects

Administration, Oral, Animals, Antimicrobial Cationic Peptides biosynthesis, Antimicrobial Cationic Peptides genetics, Bombyx genetics, Bombyx microbiology, Fat Body cytology, Fat Body immunology, Fat Body microbiology, Gene Expression, Hemocytes cytology, Hemocytes immunology, Hemocytes microbiology, Hemolymph cytology, Hemolymph immunology, Hemolymph microbiology, Hot Temperature, Insect Proteins biosynthesis, Insect Proteins genetics, Larva genetics, Larva immunology, Larva microbiology, Lipopolysaccharides pharmacology, Neuropeptides biosynthesis, Neuropeptides genetics, Pseudomonas aeruginosa chemistry, Pseudomonas aeruginosa immunology, Adaptive Immunity, Antimicrobial Cationic Peptides immunology, Bombyx immunology, Insect Proteins immunology, Neuropeptides immunology

Abstract

In the present study, we examined whether microorganisms collaterally ingested by insects with their food activate the innate immune system to confer systemic resistance against subsequent bacterial invasion. Silkworms orally administered heat-killed Pseudomonas aeruginosa cells showed resistance against intra-hemolymph infection by P. aeruginosa. Oral administration of peptidoglycans, cell wall components of P. aeruginosa, conferred protective effects against P. aeruginosa infection, whereas oral administration of lipopolysaccharides, bacterial surface components, did not. In silkworms orally administered heat-killed P. aeruginosa cells, P. aeruginosa growth was inhibited in the hemolymph, and mRNA amounts of the antimicrobial peptides cecropin A and moricin were increased in the hemocytes and fat body. Furthermore, the amount of paralytic peptide, an insect cytokine that activates innate immune reactions, was increased in the hemolymph of silkworms orally administered heat-killed P. aeruginosa cells. These findings suggest that insects sense bacteria present in their food by peptidoglycan recognition, which activates systemic immune reactions to defend the insects against a second round of infection.

Published

2015

145. Economic analysis of Royalactin production under uncertainty: Evaluating the effect of parameter optimization.

Author

Torres-Acosta MA, Aguilar-Yañez JM, Rito-Palomares M, and Titchener-Hooker NJ

Subjects

Animals, Bees, Monte Carlo Method, Sensitivity and Specificity, Software, Uncertainty, Fermentation, Glycoproteins biosynthesis, Insect Proteins biosynthesis, Models, Economic, Pichia metabolism

Abstract

Royalactin is a protein with several different potential uses in humans. Research, in insects and in mammalian cells, has shown that it can accelerate cell division and prevent apoptosis. The method of action is through the use of the epidermal growth factor receptor, which is present in humans. Potential use in humans could be to lower cholesterolemic levels in blood, and to elicit similar effects to those seen in bees, e.g., increased lifespan. Mass production of Royalactin has not been accomplished, though a recent article presented a Pichia pastoris fermentation and recovery by aqueous two-phase systems at laboratory scale as a possible basis for production. Economic modelling is a useful tool with which compare possible outcomes for the production of such a molecule and in particular, to locate areas where additional research is needed and optimization may be required. This study uses the BioSolve software to perform an economic analysis on the scale-up of the putative process for Royalactin. The key parameters affecting the cost of production were located via a sensitivity analysis and then evaluated by Monte Carlo analysis. Results show that if titer is not optimized the strategy to maintain a low cost of goods is process oriented. After optimization of this parameter the strategy changes to a product-oriented and the target output becomes the critical parameter determining the cost of goods. This study serves to provide a framework for the evaluation of strategies for future production of Royalactin, by analyzing the factors that influence its cost of manufacture., (© 2015 The Authors Biotechnology Progress published by Wiley Periodicals, Inc. on behalf of American Institute of Chemical Engineers.)

Published

2015

146. Studying translational control in non-model stressed organisms by polysomal profiling.

Author

Bernabò P, Lunelli L, Quattrone A, Jousson O, Lencioni V, and Viero G

Subjects

Animals, Chironomidae genetics, Gene Expression Regulation, HSP70 Heat-Shock Proteins genetics, Hot Temperature, Insect Proteins genetics, Larva metabolism, Polyribosomes genetics, Polyribosomes metabolism, RNA, Messenger genetics, RNA, Messenger metabolism, Ribosomal Proteins biosynthesis, Ribosomal Proteins genetics, Stress, Physiological, Chironomidae metabolism, HSP70 Heat-Shock Proteins metabolism, Insect Proteins biosynthesis

Abstract

In stressed organisms, strategic proteins are selectively translated even if the global process of protein synthesis is compromised. The determination of protein concentrations in tissues of non-model organisms (thus with limited genomic information) is challenging due to the absence of specific antibodies. Moreover, estimating protein levels quantifying transcriptional responses may be misleading, because translational control mechanisms uncouple protein and mRNAs abundances. Translational control is increasingly recognized as a hub where regulation of gene expression converges to shape proteomes, but it is almost completely overlooked in molecular ecology studies. An interesting approach to study translation and its control mechanisms is the analysis of variations of gene-specific translational efficiencies by quantifying mRNAs associated to ribosomes. In this paper, we propose a robust and streamlined pipeline for purifying ribosome-associated mRNAs and calculating global and gene-specific translation efficiencies from non-model insect's species. This method might found applications in molecular ecology to study responses to environmental stressors in non-model organisms., (Copyright © 2015 Elsevier Ltd. All rights reserved.)

Published

2015

147. AealRACK1 expression and localization in response to stress in C6/36 HT mosquito cells.

Author

González-Calixto C, Cázares-Raga FE, Cortés-Martínez L, Del Angel RM, Medina-Ramírez F, Mosso C, Ocádiz-Ruiz R, Valenzuela JG, Rodríguez MH, and Hernández-Hernández Fde L

Subjects

Animals, Cell Line, Aedes metabolism, Gene Expression Regulation, Insect Proteins biosynthesis, Receptors, Cytoplasmic and Nuclear biosynthesis, Signal Transduction

Abstract

The Receptor for Activated C Kinase 1 (RACK1), a scaffold protein member of the tryptophan-aspartate (WD) repeat family, folds in a seven-bladed β-propeller structure that permits the association of proteins to form active complexes. Mosquitoes of the genus Aedes sp., are vectors of virus producing important diseases such as: dengue, chikungunya and yellow fever. Based on the highly conserved gene sequence of AeaeRACK1 of the mosquito Aedes aegypti we characterized the mRNA and protein of the homologous AealRACK1 from the Ae. albopictus-derived cell line C6/36 HT. Two protein species differing in MW/pI values were observed at 35kDa/8.0 and 36kDa/6.5. The behavior of AealRACK1 was studied inducing stress with serum deprivation and the glucocorticoid dexamethasone. Both stressors induced increase of the expression of AealRACK1 mRNA and proteins. In serum-deprived cells AealRACK1 protein was located cortically near the plasma membrane in contrast to dexamethasone-treated cells where the protein formed a dotted pattern in the cytoplasm. In addition, 33 protein partners were identified by immunoprecipitation and mass spectrometry. Most of the identified proteins were ribosomal, involved in signaling pathways and stress responses. Our results suggest that AealRACK1 in C6/36 HT cells respond to stress increasing its synthesis and producing phosphorylated activated form., Biological Significance: Insect cells adapt to numerous environmental stressors, including chemicals and invasion of pathogenic microorganisms among others, coordinating cellular and organismal responses. Individual cells sense the environment using receptors that trigger signaling pathways that regulate expression of specific effector proteins and/or cellular responses as movement or secretion. In the coordination of responses to stress, scaffold proteins are pivotal molecules that recruit other proteins forming active complexes. The Receptor for Activated C Kinase 1 (RACK1) is the best studied member of the conserved tryptophan-aspartate (WD) repeat family. RACK1 folds in a seven-bladed β-propeller structure and it could be activated during stress, participating in different signaling pathways. The presence and activities of RACK1 in mosquitoes had not been documented before, in this work the molecule is demonstrated in an Aedes albopictus-derived cell line and its reaction to stress is observed under the effect of serum deprivation and the presence of glucocorticoid analog dexamethasone, a chemical used to cause stress in vitro., (Copyright © 2014 Elsevier B.V. All rights reserved.)

Published

2015

148. Adaptive regulation of digestive serine proteases in the larval midgut of Helicoverpa armigera in response to a plant protease inhibitor.

Author

Kuwar SS, Pauchet Y, Vogel H, and Heckel DG

Subjects

Animals, Chymotrypsin biosynthesis, Digestive System enzymology, Gene Expression Profiling, Larva drug effects, Larva enzymology, Larva growth & development, Moths drug effects, Moths growth & development, Trypsin biosynthesis, Insect Proteins biosynthesis, Moths enzymology, Plant Proteins pharmacology, Protease Inhibitors pharmacology, Serine Endopeptidases biosynthesis, Serine Proteases biosynthesis, Glycine max chemistry

Abstract

Protease inhibitors (PIs) are direct defenses induced by plants in response to herbivory. PIs reduce herbivore digestive efficiency by inhibiting insects' digestive proteases; in turn insects can adapt to PIs by generally increasing protease levels and/or by inducing the expression of PI-insensitive proteases. Helicoverpa armigera, a highly polyphagous lepidopteran insect pest, is known for its ability to adapt to PIs. To advance our molecular and functional understanding of the regulation of digestive proteases, we performed a comprehensive gene expression experiment of H. armigera exposed to soybean Kunitz trypsin inhibitor (SKTI) using a custom-designed microarray. We observed poor larval growth on the SKTI diet until 24 h, however after 48 h larvae attained comparable weight to that of control diet. Although initially the expression of several trypsins and chymotrypsins increased, eventually the expression of some trypsins decreased, while the number of chymotrypsins and their expression increased in response to SKTI. Some of the diverged serine proteases were also differentially expressed. The expression of serine proteases observed using microarrays were further validated by qRT-PCR at different time points (12, 24, 48, 72 and 96 h) after the start of SKTI ingestion. There were also large changes in transcriptional patterns over time in the control diet. Carbohydrate metabolism and immune defense genes were affected in response to SKTI ingestion. Enzyme assays revealed reduced trypsin-specific activity and increased chymotrypsin-specific activity in response to SKTI. The differential regulation of trypsins and chymotrypsins at the transcript and protein levels accompanying a rebound in growth rate indicates that induction of SKTI-insensitive proteases is an effective strategy of H. armigera in coping with this protease inhibitor in its diet., (Copyright © 2015 Elsevier Ltd. All rights reserved.)

Published

2015

149. Parallel epigenomic and transcriptomic responses to viral infection in honey bees (Apis mellifera).

Author

Galbraith DA, Yang X, Niño EL, Yi S, and Grozinger C

Subjects

Animals, Bees genetics, Bees virology, Gene Expression Profiling, Insect Proteins genetics, Picornaviridae genetics, Picornaviridae Infections genetics, Bees metabolism, Epigenesis, Genetic, Insect Proteins biosynthesis, Picornaviridae metabolism, Picornaviridae Infections metabolism, Transcriptome

Abstract

Populations of honey bees are declining throughout the world, with US beekeepers losing 30% of their colonies each winter. Though multiple factors are driving these colony losses, it is increasingly clear that viruses play a major role. However, information about the molecular mechanisms mediating antiviral immunity in honey bees is surprisingly limited. Here, we examined the transcriptional and epigenetic (DNA methylation) responses to viral infection in honey bee workers. One-day old worker honey bees were fed solutions containing Israeli Acute Paralysis Virus (IAPV), a virus which causes muscle paralysis and death and has previously been associated with colony loss. Uninfected control and infected, symptomatic bees were collected within 20-24 hours after infection. Worker fat bodies, the primary tissue involved in metabolism, detoxification and immune responses, were collected for analysis. We performed transcriptome- and bisulfite-sequencing of the worker fat bodies to identify genome-wide gene expression and DNA methylation patterns associated with viral infection. There were 753 differentially expressed genes (FDR<0.05) in infected versus control bees, including several genes involved in epigenetic and antiviral pathways. DNA methylation status of 156 genes (FDR<0.1) changed significantly as a result of the infection, including those involved in antiviral responses in humans. There was no significant overlap between the significantly differentially expressed and significantly differentially methylated genes, and indeed, the genomic characteristics of these sets of genes were quite distinct. Our results indicate that honey bees have two distinct molecular pathways, mediated by transcription and methylation, that modulate protein levels and/or function in response to viral infections.

Published

2015

150. Tweedle cuticular protein BmCPT1 is involved in innate immunity by participating in recognition of Escherichia coli.

Author

Liang J, Wang T, Xiang Z, and He N

Subjects

Acute-Phase Proteins metabolism, Amino Acid Sequence, Animals, Bombyx genetics, Bombyx immunology, Carrier Proteins metabolism, Escherichia coli, Gene Expression, Hemocytes, Hemolymph immunology, Hemolymph metabolism, Insect Proteins biosynthesis, Intercellular Signaling Peptides and Proteins, Membrane Glycoproteins metabolism, NF-kappa B genetics, NF-kappa B metabolism, Peptidoglycan, Protein Processing, Post-Translational, Proteins, Transcription Factors genetics, Transcription Factors metabolism, Transcriptional Activation physiology, Bombyx metabolism, Immunity, Innate, Insect Proteins genetics

Abstract

Bombyx mori, a lepidopteran insect, is one of the earliest models for pattern recognition of Gram-negative bacteria, which may induce the IMD pathway for production of antibacterial peptides. So far, several recognition proteins have been reported in B. mori. However, the connection between pattern recognition of Gram negative bacteria and activation of BmRelish1, a transcription factor controlled by the IMD pathway remains largely unknown. In the present study, we identify BmCPT1, a cuticle protein bearing a Tweedle domain. Its gene expression is co-regulated by NF-kappaB and juvenile hormone signals. BmCPT1 is induced by Escherichia coli in fat bodies and hemocytes, but is constitutively expressed in the epidermis. In vitro binding assays indicate that BmCPT1 protein recognizes and binds to E. coli peptidoglycan. Post-transcriptionally modified BmCPT1 in the hemolymph binds to E. coli cells through interactions with peptidoglycan recognition protein-5 (BmPGRP5) and lipopolysaccharide binding protein (BmLBP). Transgenic overexpression of BmCPT1 causes the upregulated expression of BmRelish1 and clear induction of two gloverin genes. Therefore, BmCPT1 may work along with BmPGRP-S5 and BmLBP to recognize E. coli in the hemolymph and indirectly activate BmRelish1 to induce antimicrobial peptide synthesis., (Copyright © 2014. Published by Elsevier Ltd.)

Published

2015