Exogenous estradiol improves shell strength in laying hens at the end of the laying period

Wistedt, Anna; Ridderstråle, Yvonne; Wall, H.; Holm, Lena

doi:10.1186/1751-0147-56-34

Cited by 30 publications

(17 citation statements)

References 36 publications

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“…Interestingly, similar to MT2, GnIHR was also found to be expressed in both the thecal and granulosa layers32. It has been reported that E2 secretion and GnIHR expression regulate egg production and quality33343536. GnIHR is mainly expressed in the pituitary.…”

Section: Discussionmentioning

confidence: 89%

Melatonin implantation improved the egg-laying rate and quality in hens past their peak egg-laying age

Yang

Zhu

et al. 2016

Sci Rep

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The egg-laying rates of hens approximately 470 days of age exhibited a positive correlation to blood melatonin levels. The hens with an egg-laying rate <30%, 30~90% and ≥90% had blood melatonin levels of 5.8 ± 2.6, 74.0 ± 32.9 and 445.9 ± 115.3 ng/ml, respectively. When 10 mg of melatonin was implanted into the hens at 300, 360, 470 and 550 days of age, the egg-laying rates increased 4.63 ± 0.46%, 8.38 ± 1.45%, 4.93 ± 0.85% and 7.93 ± 0.91%, respectively, compared to that of the controls. Melatonin implantation in hens at 300–470 days of age was observed to enhance egg production and reduce the rate of appearance of sharpei eggs. Melatonin (10 mg) implanted in hens 360 days of age did not influence the blood levels of progesterone (P4) or the gene expression levels of ovarian follicle stimulating hormone receptor (FSHR), luteinizing hormone receptor (LHR), oestradiol receptor alpha (ERα), superoxide dismutase 2 (SOD2) or melatonin receptor 1 (MT1). In contrast, melatonin significantly elevated the serum oestradiol-17β (E2) content, down-regulated the gene expression of gonadotropin-inhibitory hormone receptor (GnIHR), and enhanced the expression of melatonin receptor 2 (MT2). This result indicates that the improved egg-laying rate by melatonin was the result of increased serum oestradiol and decreased ovarian GnIHR. These alterations may be mediated by MT2 activation.

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Section: Discussionmentioning

confidence: 89%

Melatonin implantation improved the egg-laying rate and quality in hens past their peak egg-laying age

Yang

Zhu

et al. 2016

Sci Rep

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“…Some reports demonstrated the paradoxical role of estradiol in affecting eggshell quality. For example, injecting pellets of estradiol 3-benzoate subcutaneously in laying hens was reported to increase shell thickness and improve shell deformation (Wistedt et al, 2014). In contrast, an injection of 0.5-5 ng g −1 diethylstilbestrol (DES) into the yolk before incubation decreased later egg weight, shell strength and thickness, which accompanied abnormal development of the oviducts after sexual maturation (Kamata et al, 2009).…”

Section: Discussionmentioning

confidence: 99%

Dietary calcium deficiency in laying ducks impairs eggshell quality by suppressing the process of shell biomineralization

Chen

Zhao

Tian

et al. 2015

Journal of Experimental Biology

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The objective of this study was to determine the effects of dietary calcium deficiency on the process of shell formation. Four hundred and fifty female ducks (Anas platyrhynchos) at 22 weeks were randomly assigned to three groups. Ducks were fed one of two calcium-deficient diets (containing 1.8% or 0.38% calcium, respectively) or a calcium-adequate control diet (containing 3.6% calcium) for 67 days (depletion period) and then all ducks were fed a calcium-adequate diet for an additional 67 days (repletion period). Compared with the calcium-adequate control, the average shell thickness, egg shell weight, breaking strength, mammillae density and mammillary knob thickness of shell from ducks that consumed the diet with 0.38% calcium were significantly decreased (P<0.05) during the depletion period, accompanied by reduced tibia quality. The mRNA expression of both secreted phosphoprotein 1 (SPP1) and carbonic anhydrase 2 (CA2) in the uterus was decreased after feeding calcium-deficient diets (1.8% or 0.38% calcium). mRNA transcripts of calbindin 1 (CALB1), an important protein responsible for calcium transport, and the matrix protein genes ovocalyxin-32 (OCX-32) and ovocleidin-116 (OC-116) were reduced in ducks fed 0.38% calcium but not 1.8% calcium. Plasma estradiol concentration was decreased by both of the calciumdeficient diets (P<0.05). The impaired shell quality and suppressed functional proteins involved in shell formation could be reversed by repletion of dietary calcium. The results of the present study suggest that dietary calcium deficiency negatively affects eggshell quality and microarchitecture, probably by suppressing shell biomineralization.

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“…Dick et al (2003) found that in membrane vesicle preparations from renal distal tubule cells 17beta estradiol, testosterone and dihydrotestosterone increased PMCA activity after 24 h, but not after 1 or 5 h of exposure. In a study on the effects of exogenous estradiol on shell strength in laying hens, Wistedt et al (2014) observed that the hormone had no regulatory effect on PMCA activity in the duodenum and shell gland. If one thinks about it, PMCAs are not the best site for controlling Ca 2+ -extrusion from cells if they would pump the excess Ca 2+ into the blood, thereby increasing the toxic transmembrane Ca 2+ -gradient for all cells.…”

Section: Pmcasmentioning

confidence: 97%

The essence of female–male physiological dimorphism: Differential Ca2+-homeostasis enabled by the interplay between farnesol-like endogenous sesquiterpenoids and sex-steroids? The Calcigender paradigm

Loof

2015

General and Comparative Endocrinology

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Ca(2+) is the most omnipresent pollutant on earth, in higher concentrations a real threat to all living cells. When [Ca(2+)]i rises above 100 nM (=resting level), excess Ca(2+) needs to be confined in the SER and mitochondria, or extruded by the different Ca(2+)-ATPases. The evolutionary origin of eggs and sperm cells has a crucial, yet often overlooked link with Ca(2+)-homeostasis. Because there is no goal whatsoever in evolution, gametes did neither originate "with the purpose" of generating a progeny nor of increasing fitness by introducing meiosis. The explanation may simply be that females "invented the trick" to extrude eggs from their body as an escape strategy for getting rid of toxic excess Ca(2+) resulting from a sex-hormone driven increased influx into particular cells and tissues. The production of Ca(2+)-rich milk, seminal fluid in males and all secreted proteins by eukaryotic cells may be similarly explained. This view necessitates an upgrade of the role of the RER-Golgi system in extruding Ca(2+). In the context of insect metamorphosis, it has recently been (re)discovered that (some isoforms of) Ca(2+)-ATPases act as membrane receptors for some types of lipophilic ligands, in particular for endogenous farnesol-like sesquiterpenoids (FLS) and, perhaps, for some steroid hormones as well. A novel paradigm, tentatively named "Calcigender" emerges. Its essence is: gender-specific physiotypes ensue from differential Ca(2+)-homeostasis enabled by genetic differences, farnesol/FLS and sex hormones. Apparently the body of reproducing females gets temporarily more poisoned by Ca(2+) than the male one, a selective benefit rather than a disadvantage.

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Exogenous estradiol improves shell strength in laying hens at the end of the laying period

Cited by 30 publications

References 36 publications

Melatonin implantation improved the egg-laying rate and quality in hens past their peak egg-laying age

Melatonin implantation improved the egg-laying rate and quality in hens past their peak egg-laying age

Dietary calcium deficiency in laying ducks impairs eggshell quality by suppressing the process of shell biomineralization

The essence of female–male physiological dimorphism: Differential Ca2+-homeostasis enabled by the interplay between farnesol-like endogenous sesquiterpenoids and sex-steroids? The Calcigender paradigm

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