Photoreception and Photoreceptors

Candidate DBPs for Photo-Induced Sexual Maturation

Since the first discovery of DBPs, new opsin families have been identified in the hypothalamus. The recent annotation of opsin sequences within the chicken genome has allowed for the identification of five opsin family categories under which all opsins can be classified, including OPN1, OPN3, OPN4, OPN5, and retinal G-protein coupled receptors (RGR; Table 1). The family of OPN1 includes VA-opsin, expressed in the hypothalamus and pineal gland, as well as rhodopsin, expressed in the retina and pineal gland (Foster et al., 1985, 1994; Halford et al., 2009; Davies et al., 2012). Conversely, members from the OPN3 family consist of teleost multiple tissue opsins (TMTs) found in the cerebellum, retina and the PVN of the hypothalamus, and encephalopsins found in the cerebellum as well as the thalamic nuclei (Kato et al., 2016), suggesting this family does not play a role in reproductive control due to its localization outside the light-sensitive regions associated with reproduction. Similarly, with RGR expressed in the retina and pineal gland rather than the brain, evidence supports a role in circadian rhythm and vision rather than reproduction (Díaz et al., 2017). Meanwhile, two additional candidates, OPN4 and OPN5 were identified within various photosensitive regions throughout the hypothalamus (Chaurasia et al., 2005; Kang et al., 2010; Nakane and Yoshimura, 2010; Ohuchi et al., 2012), with OPN4 also expressed in the pineal gland (Chaurasia et al., 2005; Kang et al., 2010), and the retina (Tomonari et al., 2005). Thus, based on location, OPN1, OPN4, and OPN5 appear to be the best candidates to act as mediators of photoperiod on reproduction and are further discussed below.

TABLE 1

Summary of the candidates for deep brain photoreception.

	Opsins	Wavelengths		DBP
Family	consolidated	(nm)	Expression	criteria
				1	2	3	4
OPN1	Vertebrate ancient (VA) Opsins	450–520	Pineal gland Hypothalamus
	Rhodopsin	480–495	Pineal gland Skin Retina	x
	Pinopsins	480–540	Pineal gland	x
OPN3	Teleost multiple tissue (TMT) opsins	450–470	Cerebellum Retina Paraventricular nucleus	x		x	x
	Encephalopsins		Cerebellum Thalamic nuclei	x		x	x
OPN4	Melanopsins	410–480	Hypothalamus Pineal gland Retina			x	x
OPN5	Neuropsin	350–470	Hypothalamus			x	x
RGR	Retinal G protein-coupled receptors	470–490	Retina	x		x	x
	Peropsins		Pineal gland	x		x	x

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The five families of opsins broken down into their components, along with their associated wavelength of spectral absorption (nm), the signaling pathway they utilized and where they are expressed in the chicken. Wavelengths indicated in BOLD are within the 492 nm maximum spectral absorption hypothesized to be associated with reproduction. The deep brain photoreceptor (DBP) criteria refer to (1) Explicit expression in photosensitive regions of the brain; (2) Physiological capability of the molecule to signal light as an opsin/vitamin A-based photopigment; (3) Appropriate maximum spectral absorption, predicted to be ~492 nm; and (4) Correspond to the maximum photon capture and spectrum of available light within the hypothalamus (Foster and Follett, 1985; Davies et al., 2012).

Peroxisome Proliferator-Activated Receptor Gamma (PPAR-γ)

Peroxisome Proliferator-activated Receptor Gamma is an important regulator of lipogenesis and adipogenesis in mammals (Luquet et al., 2004). PPAR-γ is a member of the nuclear hormone receptor superfamily, binding to the peroxisome proliferator-response element, located in the promotor region of genes directly associated with glucose, and lipid homeostasis (Straus and Glass, 2001). It is highly expressed in all pituitary secretory cells in humans (Bogazzi et al., 2005), as well as adipose tissue of broilers where it plays a major role on fat deposition (Meng et al., 2005; Wang et al., 2008; Zhang et al., 2015). In fact, as this factor is associated specifically with the differentiation of adipocytes and lipid accumulation, it has been linked to NPY which is itself involved in the synthesis of preadipocytes in chicken adipose tissue in vitro (Zhang et al., 2015; Shipp et al., 2016). Thus, these studies suggest that PPAR-γ may be a link between the regulation of appetite and body composition. Additionally, elevated expression of this transcription factor has been observed in the liver of broilers selected for fatness in comparison to lean birds (Larkina et al., 2011; Zhang et al., 2015), further demonstrating the ability of this factor to divert nutrients to adipose deposition. Interestingly, variations in PPAR-γ levels have also been associated with genotype, age, and sex (Meng et al., 2005; Sato et al., 2009). In the laying hen, PPAR-γ has been detected in various tissues including the brain, liver and ovary (Sato et al., 2004; Meng et al., 2005; Hojo et al., 2006; Ojano-Dirain et al., 2007; Wang et al., 2012), suggesting a possible role in the control of reproduction. A 23-fold increase in PPAR-γ mRNA was observed in the liver of layers administered high doses of exogenous E₂ (Lee et al., 2010). This was associated with a corresponding increase in fatty acids, triacylglycerol, and an accumulation of hepatic lipids (Sato et al., 2009; Lee et al., 2010), thus implicating PPAR-γ in the formation of yolk precursors in the liver, an organ under the control of E₂ (Deeley et al., 1975). If PPAR-γ upregulates the expression of MRAP, as previously discussed, this would suggest that E₂, through its ability to directly trigger the upregulation of PPAR-γ, has the ability to activate the melanocortin system, diverting energy expenditure from growth to reproduction, linking sex steroids, and energy homeostasis. As a matter of fact, this has also led to the hypothesis that PPAR-γ may play a role in the control of egg production overall, as demonstrated through higher expression levels in high producing laying hens compared to low producing lines (Chen et al., 2010). Beyond egg formation, PPAR-γ has also been suggested to play a role in the control of gonadotropins, with one study hypothesizing that chicken prostaglandin-D synthase protein has the ability to regulate LH-β transcription via PPAR signaling pathways (Chen et al., 2010). Whether this is a direct or indirect effect is not known.

Adiponectin

Adiponectin is a cytokine predominantly secreted by the adipose tissue with a significant role in lipid and carbohydrate metabolism in mammals (Kadowaki and Yamauchi, 2005). In addition to the breakdown of fatty acids, adiponectin increases insulin sensitivity in mice (Yamauchi et al., 2002), with involvements in energy balance and body weight (Fruebis et al., 2001; Yamauchi et al., 2001). In the chicken, while adiponectin is highly expressed in adipose tissue, it is also expressed in the liver, anterior pituitary, hypothalamus, kidney, skeletal muscle, and ovary (Maddineni et al., 2005; Chabrolle et al., 2007). Plasma concentrations of adiponectin have been shown to decline in broiler chicks between 4 to 8 woa, corresponding to an increase in body weight and a 2-fold increase in abdominal fat pad during this time (Maddineni et al., 2005). While a decline in plasma adiponectin was not observed in birds fasted for 48 h (Hendricks et al., 2009), mRNA levels were found to significantly decline in adipose, liver and anterior pituitary, with other tissues, such as the hypothalamus, remaining unaffected (Maddineni et al., 2005). This implies that while expression may be altered, temporary metabolic changes have little to no influence over the short-term secretion of this hormone. Adiponectin is able to elicit its response through two receptors, AdipoR1 and AdipoR2. While AdipoR1 is primarily found in the skeletal muscle, adipose tissue and diencephalon, AdipoR2 was largely localized to the adipose tissue (Ramachandran et al., 2007), with mRNA and protein of both receptors recently found in theca and granulosa layers of ovarian follicles (Hadley et al., 2020). Signaling pathways are predicted to differ between receptors as AdipoR1 activates AMPK signaling, while AdipoR2 is believed to elicit its response through the transcription factor PPAR-α (Yamauchi et al., 2003). Regarding appetite control, in rodents adiponectin elicited an anorexigenic response through AdipoR1 and its co-localization with the leptin receptor (LEPR) in the hypothalamus, with both receptors present in NPY and POMC neurons (Guillod-Maximin et al., 2009). A similar relationship between AdipoR1 and LEPR should be investigated in avian species to determine the role of adiponectin and leptin in lipid metabolism and overall energy homeostasis within the hypothalamus. Additionally, the possibility of AdipoR1 and AdipoR2 being involved in a permissive, and/or inhibitory role with NPY and POMC should be explored in the hen, as there is the potential for integration with the melanocortin system, as discussed previously in regard to PPAR-γ. Meanwhile, AdipoR1 was upregulated by PRL, while AdipoR2 was downregulated by GH in adipose tissue of mice, (Nilsson et al., 2005), with both hormones inversely associated with adiponectin expression in both mice (Berryman et al., 2004), and humans (Mantzoros et al., 2004). Due to the critical role of these opposing hormones during the reproductive cycle of the hen, further studies should be conducted to determine a possible relationship in chickens. As reported in humans (Yamauchi et al., 2001), plasma adiponectin is negatively correlated to glycaemia in turkey hens (Diot et al., 2015), demonstrating a potential role in elevating insulin sensitivity. In the presence of elevated insulin concentrations, POMC and CART expression has been reported to elevate, while the expression of NPY is inhibited (Porte et al., 2002; Honda et al., 2007; Shiraishi et al., 2008). This is of particular interest as POMC has been found to increase in incubating Silkie hens, a period known to be associated with high PRL levels, compared to their laying counterparts (Sharp et al., 1989; Dawson, 2008; Takeda and Ohkubo, 2019). As AdipoR1 is upregulated in the presence of PRL, it would be expected that adiponectin levels would elevate during this period, yet concentrations have been observed to decline through to the end of production in turkey hens (Diot et al., 2015), requiring further investigation to determine its role throughout a production cycle.

Adiponectin is expressed exclusively in the theca layer of ovarian follicles within both broiler breeder and laying hens, with an autocrine or paracrine effect on steroidogenesis (Chabrolle et al., 2007; Hadley et al., 2020). Interestingly, in vitro treatment of porcine granulosa cells with recombinant adiponectin was found to increase steroidogenic acute regulatory protein (StAR) mRNA, along with a reduction in cytochrome P₄₅₀ aromatase, or CYP19A1 (Ledoux et al., 2006). While StAR is responsible for transporting cholesterol across the inner mitochondrial membrane in order to undergo conversion to pregnenolone (Sugawara et al., 1995; Cherradi et al., 1997), CYP19A1 converts testosterone to E₂. Altogether, this implies that regardless of the ability of adiponectin to stimulate StAR, the decline in CYP19A1 would inhibit the synthesis of E₂. Recently, granulosa cells from subsets of prehierarchal and preovulatory follicles of broiler breeder and laying hens cultured with recombinant adiponectin reported a decline in StAR mRNA abundance in all follicle groups, with the exception of F4 (Hadley et al., 2020). Additionally, the AMPK signalling pathway has been determined to be activated by adiponectin in the chicken. This AMPK pathway has been shown to differentially regulate StAR depending on the stage of follicular development (Tosca et al., 2006), suggesting that the unequivocal expression of StAR in response to adiponectin in vitro can be influenced by a variety of factors and requires further investigation. Furthermore, activation of this pathway led to an increased production of P₄, along with an elevation in StAR and CYP19A1 levels, in the absence of FSH (Tosca et al., 2006), indicating that another factor may be able to overcome the need for gonadotropin stimulation in avian species. When human recombinant adiponectin was applied to chicken granulosa cells from pre-ovulatory follicles for 36 h in culture, the expression of insulin-like growth factor-1 (IGF-1)-induced P₄ secretion in preovulatory follicles was upregulated, while LH and FSH-induced P₄ production in this same subset of follicles decreased (Chabrolle et al., 2007). This further supports the hypothesis that adiponectin is able to influence steroidogenesis within the follicular hierarchy of the chicken ovary, regardless of the status of the HPG axis. Thus, we hypothesize that adiponectin provides a mechanism through which metabolism is able to overcome the need for photostimulation during the activation of the ovary, via the stimulation of IGF-1 induced P₄ production. Further supporting the link between adiponectin and reproduction, a recent broiler breeder study showed the timing of an E₂ increase corresponded to the time during which adiponectin declined in the circulating plasma (Grandhaye et al., 2019). However, when sexually immature leghorn chickens were treated with E₂, adiponectin mRNA abundance was found to be elevated, along with the mRNA levels of AdipoR1, while P₄ treatment caused a decline in adiponectin mRNA (Hadley et al., 2020). In Huoyan geese, when ovarian granulosa cells were treated with adiponectin, a significant decline was observed in E₂, while P₄ concentration increased (Meng et al., 2019). This suggests an overall negative feedback system between adiponectin and the reproductive steroids. Furthermore, plasma adiponectin did not vary during the laying cycle, with a significant decline only found in turkey hens at the end of lay (Diot et al., 2015). Altogether, this indicates that another mechanism is utilized in order to select follicles into the preovulatory hierarchy. As adiponectin contributes to the downregulation of fat deposition (Hendricks et al., 2009; Tahmoorespur et al., 2010), which aligns with the decreased body fat percentage observed in the current commercial broiler breeder (Zuidhof et al., 2014), it is possible that these hens have elevated adiponectin levels, which may be influenced by its high mRNA expression in the liver and anterior pituitary (Maddineni et al., 2005). This would lead to the hypothesis that adiponectin is able to act in the ovary to promote IGF-1 induced P₄, rather than LH or FSH-induced P₄. This level of control must be considered to determine the effects of body weight and metabolic status on follicular development and age of first egg.

Growth Hormone (GH)

Growth hormone is produced primarily by the anterior pituitary gland under the control of hypothalamic growth hormone releasing hormone (GHRH), with additional production in a multitude of other tissues in addition to the hypothalamus (Render et al., 1995). Although initially identified as a purely somatic hormone promoting growth, a reproductive function for GH has been proposed as plasma levels correlate with the onset of lay in pullets (Williams et al., 1992), and the time of ovulation in hens (Harvey et al., 1979b). Injections of GH in immature laying hens increased ovary weight 1 week prior to maturation (Hrabia et al., 2011). However, for this to happen, it is critical that the growth hormone receptor (GH-R) be expressed within the follicles (Lebedeva et al., 2004; Hrabia et al., 2008) at that time. As GH-R expression increases in the ovary around the time of sexual maturation (Hrabia et al., 2008), it can be predicted that a similar GH effect on ovarian follicles would not occur at an earlier age. However, administration of GH increased the number of SWF (Williams et al., 1992), which not only serve as the follicular pool for the remainder of lay, but are also responsible for the production of E₂ during sexual maturation (Robinson and Etches, 1986). While GH further stimulated the release of E₂ from the pre-hierarchal follicles (Hrabia et al., 2012), a decline in this steroid hormone occurred within the hierarchy (Hrabia et al., 2014). A relationship between E₂ and GH can also be seen in the liver, which is responsive to both hormones (Stevens, 2007; Van Anes et al., 2010). GH has been linked to the elevated expression of estrogen receptor beta (ER-β) in the liver (Hrabia, 2015), suggesting an influence of GH on vitellogenesis, as demonstrated in the pigeon (Harvey et al., 1978). Interestingly, white leghorn laying hens with the sex-linked dwarf gene (dw) have been found to demonstrate a dysfunction in the GH-R gene, with a missense mutation found in the cDNA (Hull et al., 1993, 1999), reducing the GH-binding activity in the serum and liver without a complete inhibition (Hull et al., 1999). While this mutation does not appear to affect the production rate of heavy type chickens, this dw gene was found to reduce the laying rate of medium and light strains by up to 10% (Guillaume, 1976). Furthermore, these dwarf hens have been determined to be abnormally fat, with a declined ability to mobilize adipose tissue during lay (Guillaume, 1976; Burghelle-Mayeur et al., 1989), suggesting a role for body fat percentage in the ability to maintain high production rates.

At the end of the laying cycle, decreasing GH concentrations have been reported in many avian species (Scanes et al., 1979; Sharp et al., 1979; Bedrak et al., 1981). Thus, it is evident that GH has the ability to control reproduction at the level of the gonads. However, further evidence also supports an effect higher up in the HPG axis as GH-containing neurons are located throughout the hypothalamus of both turkey hens and ring doves, specifically in the PVN, IN, and ME (Ramesh et al., 2000), as well as the MBH in Japanese quail (Berghman et al., 1992), with expression patterns similar to PRL-containing neurons (Ramesh et al., 2000). Thus, similar to the pituitary, GH and PRL dynamics are linked in the hypothalamus. In the pituitary gland of turkey hens during the transition from egg laying to expression of incubation behaviour, PRL cells replace GH cells, as PRL becomes the predominant circulating hormone associated with the cessation of lay (Ramesh et al., 1996). As the hen begins to drop out of production, PRL expression in the avian brain increased (Ramesh et al., 1996), with a corresponding decline in GnRH (Saldanha et al., 1994).