Molecular Characterization and Expression of Vitellogenin Receptor from White Perch (Morone americana)

Molecular Characterization and Expression of Vitellogenin Receptor from White Perch (Morone americana)

A full-length (4021 base pair [bp]) cDNA encoding a polypeptide (844 amino acids) with a predicted mass of 93 kDa and other characteristic structural features of a vertebrate vitellogenin receptor (VgR) was isolated from a white perch ( Morone americana ) ovarian cDNA library. Northern blotting perf...

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Veröffentlicht in:Biology of reproduction 2004-06, Vol.70 (6), p.1720-1730
Hauptverfasser: HIRAMATSU, Naoshi, CHAPMAN, Robert W, LINDZEY, Jonathan K, HAYNES, Matthew R, SULLIVAN, Craig V
Format: Artikel
Sprache:eng
Schlagworte:
Alternative Splicing
Amino Acid Sequence
Animals
Base Sequence
Bass - genetics
Bass - growth & development
Bass - metabolism
Biological and medical sciences
Brackish
Cell receptors
Cell structures and functions
Cloning, Molecular
DNA, Complementary - genetics
DNA, Complementary - isolation & purification
Egg Proteins - chemistry
Egg Proteins - genetics
Female
Freshwater
Fundamental and applied biological sciences. Psychology
Gene Expression
Hormone receptors. Growth factor receptors. Cytokine receptors. Prostaglandin receptors
Molecular and cellular biology
Molecular Sequence Data
Ovary - growth & development
Ovary - metabolism
Perches - genetics
Perches - growth & development
Perches - metabolism
Receptors, Cell Surface - chemistry
Receptors, Cell Surface - genetics
Reverse Transcriptase Polymerase Chain Reaction
RNA, Messenger - genetics
RNA, Messenger - metabolism
Sequence Homology, Amino Acid
Tissue Distribution
Vertebrates: reproduction
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Zusammenfassung:A full-length (4021 base pair [bp]) cDNA encoding a polypeptide (844 amino acids) with a predicted mass of 93 kDa and other characteristic structural features of a vertebrate vitellogenin receptor (VgR) was isolated from a white perch ( Morone americana ) ovarian cDNA library. Northern blotting performed using a specific digoxygenin-labeled VgR cDNA probe revealed a distinct ∼4.1 kilobase (kb) hybridization signal in an mRNA preparation obtained from previtellogenic perch ovaries. The deduced amino acid sequence of the perch VgR was 89% and 82% identical, respectively, to that of the tilapia and rainbow trout. Because it possessed an eight-repeat ligand-binding domain (LR8) but lacked an O -linked sugar domain (−), the perch VgR was identified as a non- O -linked form of VgR (LR8−). Unlike the case in other vertebrates investigated, including tilapia and trout, no species of mRNA encoding an O -linked form of VgR (LR8+) could be detected when perch ovarian or liver mRNA reverse transcripts or cDNA libraries were screened by PCR using primer sets flanking the putative O -linked sugar domain. These novel findings call into question the assumptions that an LR8+ splice variant of the VgR always is dominantly present in somatic tissues and exists at lower levels in ovarian tissues to sequester lipoproteins distinct from Vg. A SYBR-green-based real-time reverse transcription-polymerase chain reaction assay was developed and used to quantitatively measure VgR expression in gonadal and somatic tissues, for the first time in any vertebrate. The main site of perch VgR mRNA expression was the ovary and the highest level of VgR mRNA expression was in ovaries whose largest follicles contained previtellogenic oocytes. Expression of VgR mRNA decreased with oocyte growth during vitellogenesis and was very limited in ovulated eggs. These quantitative results verify the concept that growing oocytes must extensively recycle LR8− forms of the VgR.
ISSN:0006-3363
1529-7268
DOI:10.1095/biolreprod.103.023655