Key Disulfide Bonds in an Insect Hormone Binding Protein: cDNA Cloning of a Juvenile Hormone Binding Protein of Heliothis virescens and Ligand Binding by Native and Mutant Forms

Wojtasek, Hubert; Prestwich, Glenn D.

doi:10.1021/bi00015a037

Cited by 57 publications

(55 citation statements)

References 37 publications

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“…There is also no tryptophan residue in those proteins except only one residue in B. mori JHBP. The shift of Mr observed in G. mellonella MSP was also observed in JHBPs from SDS-PAGE (Touhara et al, 1993;Kurata et al, 1994;Wojtasek and Prestwich, 1995;Vermunt et al, 2001;Parkitna et al, 2002). Based on these facts, MSP of G. mellonella could be an outer member of the JHBP family.…”

Section: Archives Of Insect Biochemistry and Physiologysupporting

confidence: 53%

“…1987; Lerro and Prestwich, 1990;Wojtasek and Prestwich, 1995;Park and Kim, 1996;Vermunt et al, 2001;Parkitna et al, 2002). Four conserved cysteins found in JHBPs were also found in MSP.…”

Section: Archives Of Insect Biochemistry and Physiologymentioning

confidence: 97%

“…Four conserved cysteins found in JHBPs were also found in MSP. These cysteins were known to be crucial in the tertiary structure and the JH binding function by making two disulfide bonds in H. virescens JHBP (Wojtasek and Prestwich, 1995). There is also no tryptophan residue in those proteins except only one residue in B. mori JHBP.…”

Section: Archives Of Insect Biochemistry and Physiologymentioning

confidence: 99%

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Cloning and expression of male‐specific protein (MSP) from the hemolymph of greater wax moth, Galleria mellonella L.

Han

Lee

Yun

et al. 2003

Arch Insect Biochem Physiol

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Male-specific protein (MSP) is a soluble protein that accumulates in high amounts in the hemolymph and other organs of adult male wax moth. The MSP was purified from adult male wax moth by gel filtration and reversed phase column chromatography, and its amino acid sequence was determined. Because of blocked N-terminus, several internal amino acid sequences of MSP were obtained by the in-gel digestion method using trypsin. RT-PCR was conducted using degenerate primers designed from the internal amino acid sequences. 5'-RACE PCR was used to obtain the complete coding region and 5'-UTR sequence. The full length MSP cDNA sequence encodes a 239 amino acid polypeptide with an 18 amino acid signal peptide. The putative mature MSP has a molecular mass of 24,317 Da and an isoelectric point (pI) of 6.00, but shows a molecular mass of 27 kDa on SDS-PAGE. Sequence alignment showed a significant similarity between MSP and juvenile hormone binding proteins (JHBPs) of several lepidopteran species, including G. mellonella.

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Section: Archives Of Insect Biochemistry and Physiologysupporting

confidence: 53%

“…1987; Lerro and Prestwich, 1990;Wojtasek and Prestwich, 1995;Park and Kim, 1996;Vermunt et al, 2001;Parkitna et al, 2002). Four conserved cysteins found in JHBPs were also found in MSP.…”

Section: Archives Of Insect Biochemistry and Physiologymentioning

confidence: 97%

Section: Archives Of Insect Biochemistry and Physiologymentioning

confidence: 99%

See 1 more Smart Citation

Cloning and expression of male‐specific protein (MSP) from the hemolymph of greater wax moth, Galleria mellonella L.

Han

Lee

Yun

et al. 2003

Arch Insect Biochem Physiol

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“…Unfortunately, the complete amino acid sequence of the G. mellonellu JHBP is not known, but the known sequences of two other JHBP, from M. sexta and H. virescens hemolymph, show the presence of one potential glycosylation site, at Asn56 in M. sextu and Asnl9 in H. virescens JHBP (Wojtasek and Prestwich, 1995). Interestingly, the Asnl9 residue was not detected during sequencing of the Nterminal peptide of H. virescens JHBP by Edman degradation (Wojtasek and Prestwich, 1995), which suggests glycosylation of this residue. The authors did not comment on this result and did not consider the possibility of glycosylation of this residue, presumably because early studies on the closely related M. sexta JHBP did not indicate a detectable content of carbohydrates (Goodman et al, 1978).…”

Section: Discussionmentioning

confidence: 99%

Evidence for Glycosylation of the Juvenile‐Hormone‐Binding Protein from Galleria mellonella Hemolymph

Duk

Krotkiewski

Forest

et al. 1996

European Journal of Biochemistry

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The juvenile-hormone-binding protein (JHBP) from Galleria mellonella hemolymph, which is a member of the high-affinity/low-molecular-mass group of JHBP proteins, was found to be glycosylated. Glycosylation was confirmed by the following evidence. Carbohydrate gas-liquid chromatography analysis of the purified JHBP preparations showed the presence of a low amount of sugars (Man and GlcNAc were the major components). The JHBP electrophoretic band blotted onto nitrocellulose was stained with GlycoTrack (a reagent kit used for the detection of protein glycosylation) and showed strong binding of concanavalin A (ConA). JHBP was fractionated on a ConA-Sepharose 4B column into ConA-bound (strongly stained with ConA) and ConA-unbound (hardly stained with ConA) portions. Both fractions showed juvenile-hormone-binding activity and were glycosylated, as revealed by staining both of them with GlycoTrack. Electrospray-ionization mass spectrometry of JHBP suggested the presence of a small amount of presumably nonglycosylated protein (24 988 Da) and five glycoforms, two of which (containing Man,GlcNAc, or Man,Fuc,GlcNAc, chain) were not bound or were weakly bound to ConA, and three (with Man,GlcNAc,, Man,Fuc, GlcNAc,, or Man,GlcNAc, chain) were present in the fraction strongly bound to ConA. In conclusion, the monosugar composition, GlycoTrack staining, ConA-binding properties and molecular mass analyses of JHBP supplied convincing evidence for its glycosylation and some information on the character of the oligosaccharide chains.

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“…The juvenile hormone-binding proteins from other insects, to which Takeout is related, are synthesized in the fat body and secreted into the hemolymph, where they are thought to carry juvenile hormone or other small lipophilic ligands to target cells (Nowock et al 1975;Glinka et al 1995;Wojtasek and Prestwich 1995). It is not known whether juvenile hormone plays any role in Drosophila male courtship behavior, but it has been shown that juvenile hormone stimulates the synthesis of accessory gland proteins (Herndon et al 1997).…”

Section: Genes and Development 2887mentioning

confidence: 99%

The Drosophila takeout gene is regulated by the somatic sex-determination pathway and affects male courtship behavior

Dauwalder¹,

Tsujimoto²,

Moss³

et al. 2002

Genes Dev.

190

254

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The Drosophila somatic sex-determination regulatory pathway has been well studied, but little is known about the target genes that it ultimately controls. In a differential screen for sex-specific transcripts expressed in fly heads, we identified a highly male-enriched transcript encoding Takeout, a protein related to a superfamily of factors that bind small lipophilic molecules. We show that sex-specific takeout transcripts derive from fat body tissue closely associated with the adult brain and are dependent on the sex determination genes doublesex (dsx) and fruitless (fru). The male-specific Doublesex and Fruitless proteins together activate Takeout expression, whereas the female-specific Doublesex protein represses takeout independently of Fru. When cells that normally express takeout are feminized by expression of the Transformer-F protein, male courtship behavior is dramatically reduced, suggesting that male identity in these cells is necessary for behavior. A loss-of-function mutation in the takeout gene reduces male courtship and synergizes with fruitless mutations, suggesting that takeout plays a redundant role with other fru-dependent factors involved in male mating behavior. Comparison of Takeout sequences to the Drosophila genome reveals a family of 20 related secreted factors. Expression analysis of a subset of these genes suggests that the takeout gene family encodes multiple factors with sex-specific functions.

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Key Disulfide Bonds in an Insect Hormone Binding Protein: cDNA Cloning of a Juvenile Hormone Binding Protein of Heliothis virescens and Ligand Binding by Native and Mutant Forms

Cited by 57 publications

References 37 publications

Cloning and expression of male‐specific protein (MSP) from the hemolymph of greater wax moth, Galleria mellonella L.

Cloning and expression of male‐specific protein (MSP) from the hemolymph of greater wax moth, Galleria mellonella L.

Evidence for Glycosylation of the Juvenile‐Hormone‐Binding Protein from Galleria mellonella Hemolymph

The Drosophila takeout gene is regulated by the somatic sex-determination pathway and affects male courtship behavior

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