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  • About
  • The Global ETD Search service is a free service for researchers to find electronic theses and dissertations. This service is provided by the Networked Digital Library of Theses and Dissertations.
    Our metadata is collected from universities around the world. If you manage a university/consortium/country archive and want to be added, details can be found on the NDLTD website.
1

Characterization of prolactin receptor in meleagris gallopavo

Zhou, Jiang Feng, 1964- January 1997 (has links)
No description available.
2

Characterization of prolactin receptor in meleagris gallopavo

Zhou, Jiang Feng, 1964- January 1997 (has links)
Prolactin receptor (PRLR) is a membrane anchored protein mediating the biological actions of prolactin. The turkey PRLR (tPRLR) cDNA was isolated and characterized. The open reading frame (ORF) of tPRLR predicted 831 amino acid residues composed of a signal peptide, an extracellular domain (ECD), a single transmembrane domain and an intracellular domain. The deduced amino acid sequence of the turkey prolactin receptor is 53.8%, 51.7%, 49.8%, 49.8%, 80.3% and 89.91% identical to that of the rabbit bovine, human, long form of the rat, pigeon and chicken PRLRs, respectively. The extracellular domain contains two homologous repeat units with 63% amino acid sequence identity to each other. The membrane-distal and membrane-proximal repeats were 53--60% and 62--70% identical to the ECDs of the mammalian PRLRs, respectively. A tPRLR transcript with a molecular size of 3 kilo nucleotides was identified and was detectable in 26 tissues examined. The pituitary gland, crop sac, duodenum and gizzard were found to express the highest levels of tPRLR mRNA among the 26 tissues. In most tissues examined there was no obvious relationship between blood levels of PRL, reproductive states and estimated concentrations of the receptor mRNA. However, in the hypothalamus, increasing blood levels of PRL were associated with decreasing levels of receptor transcripts (p < 0.05), whereas, the opposite relationship was observed in the pituitary gland (p < 0.05). The extracellular domain of tPRLR (tPRLR-ECD) was expressed as a GST fusion protein (tPRLR-ECD-GST) in E. coli. The expression of tPRLR-ECD-GST in BL21 strain yielded a protein with a molecular mass of 76 kDa. About 99% of the fusion protein was present in inclusion bodies and about 50% of the total protein in inclusion bodies was the fusion protein. The insoluble fusion protein was denatured, refolded and purified using GST affinity chromatography. The yield of the purified fusion protein was 20 mg per liter with an estimated p
3

Genetic studies of reproductive and biochemical traits in turkeys (Meleagris gallopavo) divergently selected for semen ejaculate volume

Smith, Edward J. (Edward Jude), 1961- 05 December 1991 (has links)
The genetic control of changes in unselected traits of Wrolstad Medium White turkeys divergently selected for semen ejaculate volumes (SEV) for 16 generations (G) was studied. Genetic parameters were estimated in G 10 to 14 for embryonic mortality (EM), the incidence of pipped eggs, and for total plasma cholesterol (PC) and high density lipoprotein cholesterol (HDLC) in 16-week old birds of G 15. An attempt at determining enzyme polymorphisms in the two lines was performed in G 16. A multivariate discriminant analysis procedure was established in an attempt to classify birds as low or high SEV based on fertility and incubation records in G 10 and 12. It was determined that a more reliable, yet flexible method of estimation of variance components for heritability of embryonic mortality in turkeys is a likelihood procedure. The mean heritability estimates were -.03 and .10 for embryonic mortality in the early (Days 1- 10) and late (Days 21-28), respectively. Estimates of heritability for the incidence of pipped eggs were .21 and .08 in the low and high lines respectively. Since there were no line differences (P>.05) for PC and HDLC, data was pooled from low and high SEV lines and h² was computed to be -.03 and .26, respectively. Genetic correlation among PC, HDLC, and 16 week body weight (BW) varied from .05 between PC and HDLC, .13 PC and BW and -.34 HDLC and BW. No polymorphisms were observed for the enzymes examined in the present study. The discriminant function developed to categorize birds as low or high volume semen producers, had a moderate (.55) to high (.75) hit ratio for classification of birds as low or high volume producers in G 10 and 12. It was concluded that divergence in unselected traits, embryonic mortality and the incidence of pipped eggs, in the low and high SEV lines had a negligible additive genetic control. Cholesterol, though a major intermediate in the biosynthesis of steroid hormones, in turkeys at 16 weeks of age is not a suitable biochemical marker for SEV. Although genetic control in turkeys appears to be negligible for PC, there is a moderate and significant hereditary influence on HDLC. With a misclassification rate of .30-.40, fertility and incubation records, as demonstrated here can be used to classify birds as low or high volume semen producers. / Graduation date: 1992
4

Studies on variants of prolactin in the turkey

Bédécarrats, Grégoy. January 1999 (has links)
No description available.
5

Inhibited feathering, K[I] a sex-linked dominant gene in the turkey (Meleagris gallopavo), genetics and nutrition

Zakrzewska, Elz��bieta Iwona 11 December 1995 (has links)
Graduation date: 1996
6

Studies on variants of prolactin in the turkey

Bédécarrats, Grégoy. January 1999 (has links)
Changes in the pituitary content of prolactin (PRL) and in the ratio of immunoreactive forms of PRL were measured during a reproductive cycle in turkey hens. Low levels of PRL were observed in pituitary glands from sexually immature, out-of-lay and moulting hens. Higher levels were present during the egg laying period and the highest levels were detected in hens expressing incubating behaviour. Two immunoreactive bands of apparent molecular weights of 24 and 27 kDa were visualised on western blots, corresponding to the non-glycosylated (NG-) and glycosylated (G-) forms of PRL, respectively. The percentage of G-PRL was about 60 in sexually immature and egg laying hens. In pituitaries from incubating, out-of-lay and moulting hens the percentage of G-PRL was about 70, 38 and 33, respectively. Thus, higher percentages of G-isoforms (27 kDa) were associated with high levels of total PRL and Iower percentages were associated with low levels of PRL content in the pituitary gland. Digestion of the isoforms with N-glycosidase F resulted in a single band with an apparent molecular weight of 24 kDa. Partial deglycosylation was achieved using neuraminidase, whereas digestion with O-glycosidase had no apparent effect on the isoforms. Thus, G-PRL has N-linked carbohydrates containing sialic acid. In order to study the in vitro release of the PRL isoforms, pituitary glands from turkeys at various physiological stages were stimulated by cVIP in a perifusion system. Total PRL content and the ratio of immunoreactive PRL isoforms in the perifusate were monitored. All the perifused pituitaries responded to cVIP stimulation by increasing the release of PRL. Two immunoreactive bands corresponding to the ones detected in pituitary extracts were detected by western blotting. The G-PRL (27 kDa) was predominant in samples from egg laying and incubating hens and the NG-PRL (24 kDa) was predominant in samples from out-of-lay and moulting hens. No change in the ratio of isoforms released was / A competitive reverse transcription polymerase chain reaction assay was developed in order to semi-quantify the PRL mRNA in individual pituitary glands from turkey embryos and poults. Pituitary content and plasma levels of PRL were also monitored, and the PRL isoforms present in the pituitary gland were detected. The levels of PRL mRNA remained low until five days before hatching, increased until the day of hatch, plateaued during the first three days of age and significantly increased at two weeks of age. Similar changes were observed in pituitary content and plasma concentrations of PRL which were highly correlated. Two immunoreactive bands corresponding to the NG- and G-PRL detected in adult pituitary gland were visualised on western blots. The percentage of G-PRL in pituitary glands were 31.5, 48.6, 48.0 and 56.2 at 22 and 27 days of incubation and at I and 7 days of age, respectively. Thus, higher percentages of G-PRL (27 kDa) were associated with higher levels of total PRL in the pituitary gland.
7

Sequence variation in the turkey prolactin promoter and association with incubation behaviour in female turkeys

Sotocinal, Susana G. January 2000 (has links)
No description available.
8

Cloning, characterizaion and expression of the prolactin gene in the domestic Turkey, Meleagris gallopavo

Karatzas, Constantinos N. January 1993 (has links)
A turkey prolactin (PRL) cDNA, encoding a 199 amino acid turkey PRL (tPRL), was cloned from a pituitary library. The mature PRL shared about 70% homology with mammalian PRLs and about 30% with fish PRLs. Areas of highest homology to other PRLs were located in the carboxyl terminus of the tPRL. Prolactin mRNA analyses, during the reproductive life of the turkey hen, confirmed that the high pituitary and plasma levels of PRL measured during the incubation phase are due to enhanced transcription of the PRL gene. Furthermore, tPRL mRNA levels were highly correlated with pituitary levels of tPRL. Recombinant tPRL (rctPRL), biologically and immunologically similar to pituitary tPRL, was purified from Escherichia coli cultures hosting an expression vector carrying the tPRL cDNA. Polyclonal antibodies raised against purified rctPRL behaved similar as antibodies raised against pituitary derived tPRL, in immunoblotting and immunocytochemistry experiments. Three tPRL isoforms (with estimated molecular weights of 27 kDa, 25 kDa and 24 kDa) were identified in turkey pituitary extracts. The relative proportion of the 27 kDa isoform increased while that of the 25 kDa decreased with increasing levels of total pituitary tPRL, during the reproductive life of the turkey hen. The partition of the immunoreactivity of tPRL into the three isoforms perhaps provides an additional control of the multitude functions of PRL.
9

Cloning, characterizaion and expression of the prolactin gene in the domestic Turkey, Meleagris gallopavo

Karatzas, Constantinos N. January 1993 (has links)
No description available.

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