Abstract
Substance-induced social behavior deficits dramatically worsen the clinical outcome of substance use disorders; yet, the underlying mechanisms remain poorly understood. Herein, we investigated the role for the corticotropin-releasing factor receptor 1 (CRF1) in the acute sociability deficits induced by morphine and the related activity of oxytocin (OXY)- and arginine-vasopressin (AVP)-expressing neurons of the paraventricular nucleus of the hypothalamus (PVN). For this purpose, we used both the CRF1 receptor-preferring antagonist compound antalarmin and the genetic mouse model of CRF1 receptor-deficiency. Antalarmin completely abolished sociability deficits induced by morphine in male, but not in female, C57BL/6J mice. Accordingly, genetic CRF1 receptor-deficiency eliminated morphine-induced sociability deficits in male mice. Ex vivo electrophysiology studies showed that antalarmin also eliminated morphine-induced firing of PVN neurons in male, but not in female, C57BL/6J mice. Likewise, genetic CRF1 receptor-deficiency reduced morphine-induced firing of PVN neurons in a CRF1 gene expression-dependent manner. The electrophysiology results consistently mirrored the behavioral results, indicating a link between morphine-induced PVN activity and sociability deficits. Interestingly, in male mice antalarmin abolished morphine-induced firing in neurons co-expressing OXY and AVP, but not in neurons expressing only AVP. In contrast, in female mice antalarmin did not affect morphine-induced firing of neurons co-expressing OXY and AVP or only OXY, indicating a selective sex-specific role for the CRF1 receptor in opiate-induced PVN OXY activity. The present findings demonstrate a major, sex-linked, role for the CRF1 receptor in sociability deficits and related brain alterations induced by morphine, suggesting new therapeutic strategy for opiate use disorders.
Introduction
Opiate substances often induce severe social behavior deficits, such as poor sociability, social isolation and elevated aggressiveness (Babor et al., 1976; Gerra et al., 2004). Notably, opiate-induced social behavior deficits dramatically contribute to addictive-like substance consumption, favoring the development and maintenance of opiate use disorders (OUD) (APA, 2013; Pomrenze et al., 2022). Thus, it has been hypothesized that treatments increasing positive peer relationships might considerably reduce substance-seeking and taking and ameliorate the clinical outcome of substance-dependent patients (Heilig et al., 2016; Venniro et al., 2018). However, the development of novel, effective, therapy heavily relies on a better understanding of the brain mechanisms underlying the harmful effects of substances of abuse; yet, to date the neurobiological substrates of substance-induced social behavior deficits remain largely unknown.
The corticotropin-releasing factor (CRF) system is a main orchestrator of behavioral and neuroendocrine responses to stress (Dedic et al., 2018; Koob, 2008). The CRF system might also underlie the behavioral and brain effects of substances of abuse (Koob, 2008). CRF signaling is mediated by two types of receptors, named CRF1 and CRF2 (Hauger et al., 2003). Relatively recent studies shed some light on the role for each of the two known CRF receptor types in social behavior deficits induced by repeated administration of and withdrawal from substances of abuse. For instance, genetic inactivation of the CRF2 receptor (CRF2−/−) reduced sociability deficits and vulnerability to stress associated with long-term cocaine withdrawal in male mice (Morisot et al., 2018). Moreover, genetic inactivation of the CRF1 receptor (CRF1−/−) decreased morphine withdrawal-induced sociability deficits in female mice and hostility-driven interest for a same-sex conspecific in male mice (Piccin and Contarino, 2022). Besides, extensive literature points out to the two closely related neuropeptides oxytocin (OXY) and arginine-vasopressin (AVP) as main substrates of social interaction, parenting behavior and intermale aggressiveness (Jurek and Neumann, 2018). For instance, chemogenetic activation or inhibition of OXY-expressing neurons within the paraventricular nucleus of the hypothalamus (PVN) respectively increased or decreased social approach in male mice (Resendez et al., 2020). Accordingly, social stimuli increased the activity of PVN OXY-expressing neurons, as assessed by in vivo two-photon calcium imaging (Resendez et al., 2020). In contrast, male Shank3b knock-out mice, i.e., a mouse model of autistic-like behavior, showed a marked reduction in PVN OXY-expressing neurons and decreased social approach (Peça et al., 2011; Resendez et al., 2020). Likewise OXY and AVP, CRF is largely expressed in the PVN (Jiang et al., 2018; Sawchenko et al., 1993). Interestingly, whole-cell patch-clamp studies showed that CRF- and OXY-expressing neurons are highly intermingled within the PVN, suggesting local cell-to-cell interactions (Jamieson et al., 2017). CRF might also modulate hypothalamic OXY and AVP responses to substances of abuse. For instance, long-term cocaine-withdrawn male CRF2−/−mice showed neither the stress-induced sociability deficits nor the related increased expression of OXY or AVP in the supraoptic nucleus of the hypothalamus (SON) or the PVN (Morisot et al., 2018). Thus, CRF, OXY and/or AVP systems may be potential targets of effective therapy for diseases characterized by dysfunctional social behavior, including substance use disorders. However, to date very little is known about their implication in social behavior deficits induced by substances of abuse.
Thus, herein we investigated the role for the CRF/CRF1 receptor pathway in the acute social behavior deficits following opiate administration. In particular, using the three-chamber task for sociability in mice, the role for the CRF1 receptor in sociability deficits induced by morphine was assessed by both pharmacological (i.e., the CRF1 receptor-preferring antagonist antalarmin) and genetic (i.e., the CRF1 receptor-deficient mouse model) approaches (Moy et al., 2004; Smith et al., 1998; Webster et al., 1996). Moreover, to understand CRF role in brain OXY and AVP responses to morphine, ex vivo electrophysiology studies assessed the effect of antalarmin and genetic CRF1 receptor-deficiency upon morphine-induced firing of PVN OXY- and/or AVP-immunoreactive neurons. Notably, to fully adhere to the Sex as a Biological Variable (SABV) initiative and given the well-established influence of sex upon the addictive-like properties of substances of abuse, herein male and female mice were used throughout (Becker and Koob, 2016; Clayton, 2018).
Results
Pharmacological CRF1 receptor antagonism eliminates morphine-induced sociability deficits in male, but not in female, mice
The acute effects of morphine upon social behavior were investigated using the three-chamber test for sociability in mice, as previously reported (Piccin et al., 2022). During the habituation phase of the test, male C57BL/6J mice spent similar time in the regions of interests (ROIs, side half-chambers) of the apparatus (Fig. 1A-B and Table S2). Analysis of the sociability phase revealed a pretreatment X treatment X repeated measures interaction effect (Table S2). Unlike saline-treated mice, vehicle/morphine-treated mice spent similar time in the ROIs containing the unfamiliar conspecific or the object (P=0.823), indicating sociability deficits (Fig. 1C). In contrast, antalarmin/morphine-treated mice spent more time with the unfamiliar conspecific than with the object (P<0.005), indicating unaltered sociability (Fig. 1C). Accordingly, analysis of sociability ratio revealed a pretreatment effect (F1,32=11.598, P<0.005), a treatment effect (F1,32=4.713, P<0.05) and a pretreatment X treatment interaction effect (F1,32=8.718, P<0.01). Vehicle/morphine-treated mice showed lower sociability ratio than vehicle/saline-treated mice (P<0.005, Fig. 1D). In contrast, antalarmin/morphine-treated mice did not differ from saline-treated mice (P=0.661) and showed higher sociability ratio than vehicle/morphine-treated mice (P<0.005, Fig. 1D). During the habituation phase, morphine-treated female C57BL/6J mice spent less time in the ROIs of the apparatus than saline-treated mice (P<0.0005), independently of vehicle or antalarmin pretreatment (Fig. 1E and Table S2). Moreover, analysis of the sociability phase revealed a treatment X repeated measures interaction effect but no pretreatment X treatment X repeated measures interaction effect (Table S2). Indeed, unlike saline-treated mice, morphine-treated mice spent similar time in the ROIs containing the unfamiliar conspecific or the object (P=0.259), independently of vehicle or antalarmin pretreatment (Fig. 1F). Accordingly, analysis of sociability ratio revealed no pretreatment effect (F1,21=0.035, P=0.852), a treatment effect (F1,21=8.698, P<0.01) but no pretreatment X treatment interaction effect (F1,21=0.018, P=0.894). Morphine-treated mice showed lower sociability ratio than saline-treated mice (P<0.05), independently of vehicle or antalarmin pretreatment (Fig. 1G). During the three-chamber test, morphine-treated male, but not female, mice travelled more distance than saline-treated mice (P<0.05), independently of vehicle or antalarmin pretreatment (Table S3 and Fig. S1A-B). Also, overall mice travelled more distance during the habituation than during the sociability phase (P<0.05), indicating familiarization with the test apparatus (Table S3 and Fig. S1A-B). As detailed below in the Materials and methods section, we did not statistically compare the sexes and so are limited in making direct conclusions about sex differences. However, the present results indicate a sex-linked role for the CRF1 receptor in social behavior deficits induced by morphine. Moreover, morphine effects upon sociability seemed unrelated to locomotor activity.
Pharmacological CRF1 receptor antagonism eliminates morphine-induced firing of PVN neurons in male, but not in female, mice
To investigate the neural substrates of CRF1 receptor-mediated sociability deficits induced by morphine, electrophysiology studies examined firing frequency of PVN neurons (Fig. 2A). In male C57BL/6J mice, analysis of firing frequency of all of the recorded cells (n=110) revealed a pretreatment effect (F1,106=7.894, P<0.01), a treatment effect (F1,106=13.350, P<0.0005) and a pre-treatment X treatment interaction effect (F1,106=4.208, P<0.05). Vehicle/morphine-treated mice showed higher firing frequency than vehicle/saline-treated mice (P<0.0005, Fig. 2B). In contrast, antalarmin/morphine-treated mice did not differ from saline-treated mice (P=0.552) and showed lower firing frequency than vehicle/morphine-treated mice (P<0.005, Fig. 2B). On the other hand, analysis of firing frequency of all of the recorded cells (n=93) in female C57BL/6J mice revealed no pretreatment effect (F1,89=0.049, P=0.826), a treatment effect (F1,89=20.476, P<0.0001) but no pre-treatment X treatment interaction effect (F1,89=1.045, P=0.310). Morphine similarly increased firing frequency in vehicle- or antalarmin-pretreated mice, as compared to saline-treated mice (P<0.0005, Fig. 2D). These results indicate a critical role for the CRF1 receptor in PVN neuronal activity induced by morphine in male, but not in female, mice. Notably, the sex-dependent effects of antalarmin upon neuronal firing closely mimicked the social behavior results, indicating a link between PVN activity and sociability deficits induced by morphine.
Genetic inactivation of the CRF1 receptor eliminates morphine-induced sociability deficits
The specific role for the CRF1 receptor in morphine-induced sociability deficits was further investigated using the genetic mouse model of CRF1 receptor-deficiency. We first tested n=3 CRF1+/+ and n=3 CRF1+/− male mice using the same morphine dose (2.5 mg/kg) employed in the C57BL/6J mice. However, during the whole 10-min habituation phase of the three-chamber test, all of the six morphine-treated animals remained in the central chamber of the apparatus, suggesting that the morphine dose used was relatively high. Thus, we decided to use a substantially lower morphine dose, i.e., 0.625 mg/kg (Fig. 3A). During the habituation phase, morphine (0.625 mg/kg) reduced the time spent in both ROIs of the three-chamber apparatus in CRF1+/− (P<0.05 vs. saline-treated CRF1+/− mice), but not in CRF1+/+ or CRF1−/−, male mice (Fig. 3B and Table S4). Analysis of the sociability phase revealed a genotype X treatment X repeated measures interaction effect (Table S4). Unlike saline-treated mice, morphine-treated CRF1+/+ and CRF1+/− mice spent similar time in the ROIs containing the unfamiliar conspecific or the object (P=0.873), indicating sociability deficits (Fig. 3C). In contrast, morphine-treated CRF1−/−mice spent more time with the conspecific than with the object (P<0.005), indicating unaltered sociability (Fig. 3C). Accordingly, analysis of sociability ratio revealed no genotype effect (F2,58=2.641, P=0.080), a treatment effect (F1,58=7.478, P<0.01) and a genotype X treatment interaction effect (F2,58=4.994, P<0.01). Morphine-treated CRF1+/+ mice showed lower sociability ratio than saline-treated CRF1+/+ mice (P<0.05, Fig. 3D). In contrast, morphine-treated CRF1−/−mice did not differ from saline-treated mice (P=0.819) and showed higher sociability ratio than morphine-treated CRF1+/+ and CRF1+/− mice (P<0.05, Fig. 3D). Interestingly, unlike CRF1+/+ and CRF1−/− mice, morphine-treated CRF1+/− mice almost differed from saline-treated CRF1+/− mice (P=0.065), suggesting a gene expression-dependent effect of CRF1 receptor-deficiency (Fig. 3D). During the three-chamber test, overall morphine did not affect distance travelled (Table S4). Moreover, saline-treated mice and morphine-treated CRF1+/+, but not CRF1+/− or CRF1−/−, mice travelled more distance during the habituation than during the sociability phase (P<0.05, Fig. S2 and Table S4), further indicating dissociation between the locomotor and the sociability effects of morphine. Thus, the similar results obtained with CRF1−/− and antalarmin-treated C57BL/6J male mice strengthened the notion of a key role for the CRF1 receptor in sociability deficits induced by morphine.
We then assessed the effect of morphine (0.625 mg/kg) in female CRF1 receptor-deficient mice. However, as shown in Table S5, during the habituation phase of the three-chamber test only 2/8 CRF1+/+ mice treated with saline and 2/8 CRF1+/+ mice treated with morphine visited both side chambers of the apparatus. Also, despite all saline-treated CRF1+/− mice (n=4) visited both side chambers of the apparatus, this occurred only in 3/8 CRF1+/− mice treated with morphine. Thus, we could not obtain a reliable amount of data using a reasonable number of female mice, at least under our experimental conditions and with the 0.625 mg/kg morphine dose.
CRF1 receptor-deficiency eliminates morphine-induced firing of PVN neurons
Analysis of firing frequency of PVN neurons in male CRF1 receptor-deficient mice revealed a genotype effect (F2,119=8.498, P<0.0005), a treatment effect (F1,119=31.816, P<0.0001) and a genotype X treatment interaction effect (F2,119=7.224, P<0.005). Morphine (0.625 mg/kg) increased firing frequency in CRF1+/+ (P<0.0005) and in CRF1+/− (P<0.005), but not in CRF1−/− (P=0.987), mice, as compared to same-genotype saline-treated mice (Fig. 3E). Notably, morphine-treated CRF1+/− mice showed lower or higher firing frequency than morphine-treated CRF1+/+ (P<0.05) or CRF1−/− (P<0.005) mice, respectively, indicating a CRF1 gene expression-dependent effect (Fig. 3E). These results further support an essential role for the CRF1 receptor in PVN neuronal firing induced by morphine. Moreover, the lack of morphine effects upon neuronal firing and sociability in CRF1−/− mice indicates once more a link between PVN activity and social behavior.
Pharmacological CRF1 receptor antagonism eliminates morphine-induced firing of PVN OXY-expressing neurons in male, but not in female, mice
In male C57BL/6J mice, 40 cells expressed both OXY and AVP, 49 cells expressed AVP but not OXY, 6 cells expressed OXY but not AVP and 15 cells expressed neither OXY nor AVP (Fig. 4B). Vehicle/morphine-treated mice showed higher firing frequency of OXY/AVP-expressing neurons than vehicle/saline-treated mice (P<0.0005; Fig. 4C and Table S6). In contrast, antalarmin/morphine-treated mice did not differ from saline-treated mice (P=0.782) and showed lower firing frequency than vehicle/morphine-treated mice (P<0.0005, Fig. 4C). On the other hand, morphine increased firing frequency of neurons expressing AVP, but not OXY, independently of vehicle or antalarmin pretreatment (P<0.05; Fig. 4D and Table S6). In female C57BL/6J mice, 31 cells expressed both OXY and AVP, 38 cells expressed OXY but not AVP, 7 cells expressed AVP but not OXY and 17 cells expressed neither OXY nor AVP (Fig. 4E). Morphine increased firing frequency of neurons co-expressing OXY and AVP, independently of vehicle or antalarmin pretreatment (P<0.005; Fig. 4F and Table S6). Similarly, morphine increased firing frequency of neurons expressing OXY, but not AVP, independently of vehicle or antalarmin pretreatment (P<0.005; Fig. 4G and Table S6). These results indicate a sex-specific role for the CRF1 receptor in morphine-induced firing of PVN OXY-expressing neurons, suggesting that CRF modulates brain OXY responses to substances of abuse.
Discussion
The present study demonstrates a major, sex-linked, role for the CRF1 receptor in social behavior alterations induced by morphine. Indeed, male, but not female, mice treated with the CRF1 receptor-preferring antagonist antalarmin did not show the sociability deficits induced by morphine. Accordingly, genetic inactivation of the CRF1 receptor eliminated morphine-induced sociability deficits in male mice. Antalarmin also abolished morphine-induced firing of PVN neurons in male, but not in female, mice. Consistently, in male mice CRF1 receptor-deficiency decreased morphine-induced firing of PVN neurons in a CRF1 gene expression-dependent manner. Thus, the electrophysiology results reliably mirrored the behavioral results, suggesting a link between morphine-induced neuronal activity and sociability deficits. Furthermore, in male, but not in female, mice antalarmin eliminated morphine-induced firing of PVN neurons expressing OXY, suggesting sex-specific CRF-OXY interactions.
In agreement with our previous study (Piccin et al., 2022), morphine consistently and similarly decreased sociability in male and female mice. Prior work reported sex-linked behavioral effects of opiate substances. For instance, female rats displayed greater motivation to take heroin and self-administered greater amounts of heroin or oxycodone than male rats (Cicero et al., 2003; Fulenwider et al., 2020; George et al., 2021). Moreover, female mice showed elevated heroin self-administration and increased sensitivity to the rewarding properties of morphine, as compared to male mice (Piccin et al., 2022; Towers et al., 2019). Thus, unlike other behavioral effects of opiate substances, sex might have a marginal role in opiate-induced impairment of sociability. Nevertheless, herein CRF1 receptor antagonism by antalarmin prevented morphine-induced sociability deficits in male, but not in female, mice. To date, very few studies have examined CRF role in social behavior effects of substances of abuse. For instance, genetic inactivation of the CRF2 receptor reduced sociability deficits associated with long-term cocaine withdrawal in male mice (Morisot et al., 2018). Moreover, genetic CRF1 receptor-deficiency decreased opiate withdrawal-induced sociability deficits in female mice, as assessed one week after cessation of repeated morphine administration (Piccin and Contarino, 2022). The latter findings contrast with the present results of a lack of effect of antalarmin in female mice. However, although it might be difficult to compare pharmacological and genetic studies, the possibility exists for a differential implication of the CRF1 receptor in social behavior deficits induced by acute opiate administration or following relatively long-term opiate withdrawal in female mice. Nevertheless, the present findings also bear importance for opiate-related diseases since a single morphine administration may induce long-lasting behavioral and brain alterations (Vanderschuren et al., 2001).
Genetically engineered mouse models might provide a level of molecular specificity that is rarely achieved by pharmacological tools. Thus, to specifically assess the role for the CRF1 receptor in morphine-induced sociability deficits, herein we also used CRF1 receptor-deficient mice (Smith et al., 1998). However, following preliminary experiments showing that male CRF1+/+ and CRF1+/− mice treated with morphine (2.5 mg/kg) did not explore the three-chamber apparatus, a lower morphine dose was employed. Like in C57BL/6J mice, morphine (0.625 mg/kg) reliably impaired sociability in CRF1+/+ and CRF+/− male mice, indicating that the two morphine doses used herein were suitable to compare the effect of pharmacological and genetic disruption of the CRF1 receptor. Some differences were though observed between CRF1 receptor-deficient and C57BL/6J mice treated with saline. In particular, while we did not perform direct statistical comparisons, percentage of time spent with the unfamiliar conspecific seemed higher in saline-treated CRF1+/+, CRF1+/− and CRF1−/− male mice, as compared to saline-treated C57BL/6J male mice. It is difficult to understand the factors underlying these results. However, male mice bearing a mixed (B6×129PF2/J) genetic background also showed higher sociability levels than C57BL/6J male mice (Moy et al., 2004). Thus, it is possible that the mixed (C57BL/6Jx129S4/SvJae) genetic background of the CRF1 receptor-deficient mice used herein contributed, at least in part, to increase social approach, as compared to inbred C57BL/6J mice. Nevertheless, despite the latter differences, CRF1 receptor-deficiency (CRF1−/−) completely eliminated the sociability deficits induced by morphine in male mice, further supporting the notion of an essential role for the CRF1 receptor in opiate-induced disruption of social behavior. Unlike CRF1+/+ mice, CRF1−/− mice showed sex-independent hypothalamus-pituitary-adrenal (HPA) axis deficits under basal and stressful conditions, as revealed by plasma adrenocorticotropic hormone (ACTH) and corticosterone assays (Papaleo et al., 2007; Smith et al., 1998; Timpl et al., 1998). Thus, it could be argued that the lack of morphine effects found in CRF1−/− mice was due to HPA axis alterations. However, the present antalarmin results might, at least in part, rule out the latter hypothesis. Indeed, antalarmin is a non-peptide CRF1 receptor-preferring antagonist that, upon systemic administration, readily crosses the blood-brain barrier and is behaviorally active (Zorrilla and Koob, 2010). Notably, antalarmin did affect neither basal nor stress-induced ACTH and corticosterone levels in male rats and mice (Jutkiewicz et al., 2005; Pérez-Tejada et al., 2013). Accordingly, the dose of antalarmin (20 mg/kg) used herein increased the somatic signs of morphine withdrawal without affecting plasma corticosterone (Papaleo et al., 2007). Thus, the present similar results obtained with antalarmin and CRF1−/− mice argue in favor of a marginal role for the HPA axis in CRF1 receptor-mediated sociability deficits induced by morphine.
Throughout the present studies, locomotor activity during the three-chamber test did not seem to account for the CRF1 receptor-mediated sociability deficits induced by morphine. For instance, antalarmin- and vehicle-treated male C57BL/6J mice showed similar locomotor but different sociability responses to morphine (see Fig. 1D and Fig. S1A). Moreover, morphine-treated CRF1+/− and CRF1−/− mice travelled similar distance but showed different social behavior (see Fig. 3D and Fig. S2). Finally, overall mice travelled more distance during the habituation than during the sociability phase, an effect usually observed in the three-chamber test (Piccin and Contarino, 2020a, 2020b).
The PVN is a main source of brain CRF (Sawchenko et al., 1993). Moreover, CRF release within the PVN may stimulate intra-PVN CRF1 receptor-expressing neurons (Jiang et al., 2019, 2018). Thus, to further explore the mechanisms of CRF1 receptor-mediated sociability deficits, we examined neuronal responses to morphine in the PVN. We found that morphine consistently elevated the firing frequency of PVN neurons in male and female C57BL/6J mice, and in male CRF1+/+ and CRF1+/− mice. Acute morphine treatment increases CRF level in the hypothalamus and HPA axis activity (Buckingham, 1982; Ignar and Kuhn, 1990). Thus, although herein we did not examine CRF expression, it is likely that morphine increased PVN CRF activity. We also show that CRF1 receptor antagonism by antalarmin completely eliminated morphine-induced PVN neuronal firing in male, but not in female, mice. Likewise, in male mice genetic inactivation of the CRF1 receptor decreased morphine-induced PVN neuronal firing in a CRF1 gene expression-dependent manner. Sex-linked differences in brain distribution and activity of the CRF system might underlie the latter findings. For instance, female rats displayed higher CRF expression in the PVN and in the central nucleus of the amygdala (CeA), as compared to male rats (Iwasaki-Sekino et al., 2009). However, using a CRF1 reporter mouse line maintained on a C57BL/6 background, studies showed higher levels of the CRF1 receptor in the PVN of adult (2 months) and old (20-24 months) male mice, as compared to adult and old female mice (Rosinger et al., 2019). Moreover, adult gonadectomy (6 weeks) decreased PVN CRF1 receptor-immunoreactive cells in male, but not in female, mice, indicating a sex-linked modulation of CRF1 receptors by gonadal hormones (Rosinger et al., 2019). Thus, based on the latter findings, it is possible that elevated PVN CRF1 receptor levels in male mice, as compared to female mice, contributed to the sex-linked behavioral and brain effects of antalarmin reported herein.
The present immunohistochemistry studies showed that, in male and female C57BL/6J mice, approximately half of the patched PVN cells expressed both OXY and AVP. However, in male mice a relatively large portion of the stained cells expressed AVP, but not OXY. In net contrast, in female mice a large portion of the stained cells expressed OXY, but not AVP. The latter sex differences resonate with previous studies. Indeed, AVP- or OXY-positive neurons were shown to be more numerous in the PVN of male or female animals, respectively, in a variety of species, including humans (Dumais and Veenema, 2016). Interestingly, herein morphine disrupted sociability but increased the firing frequency of PVN neurons expressing OXY and/or AVP. At first glance, these results might seem at odds with the alleged prosocial role for OXY systems. However, PVN OXY neurons extensively project to several brain regions where they may differentially modulate social behavior in a brain site-specific manner (Jurek and Neumann, 2018). For instance, genetically-driven activation or inhibition of PVN OXY neurons projecting to the ventral tegmental area respectively increased or decreased social interaction in male mice (Hung et al., 2017). In contrast, OXY infusion into the bed nucleus of the stria terminalis (BNST) dose-dependently decreased social approach in both male and female California mice (Duque-Wilckens et al., 2020). Moreover, both pharmacological antagonism of OXY receptors and genetic inhibition of OXY synthesis within the BNST attenuated social defeat stress-induced reduction of social interaction in female California mice, further indicating a negative modulation of social behavior by BNST OXY activity (Duque-Wilckens et al., 2020, 2018). In addition, stressful events strongly activate brain OXY systems (Jurek and Neumann, 2018). For instance, male rats exposed to the forced swim or the tail suspension stressor showed increased OXY peptide levels in several brain regions, including the PVN and the SON (Yan et al., 2014). Notably, intracerebroventricular injection of an OXY receptor antagonist dose-dependently increased stress-induced immobility, suggesting that OXY activity served to cope with stress (Yan et al., 2014). Acute morphine administration may elicit a stress-like state, as revealed by elevated CRF mRNA in the CeA and HPA axis activity in male rats (Ignar and Kuhn, 1990; Maj et al., 2003). Within this framework, the present results of morphine-induced firing of PVN OXY-positive neurons suggest the presence of a stress-like state, which may disrupt social behavior. Thus, morphine may activate brain CRF systems which, via CRF1 receptors, may increase the activity of PVN OXY neurons in order to counteract stress effects. Accordingly, CRF1 receptor mRNA and OXY mRNA were shown to co-localize in PVN neurons in male rats (Arima and Aguilera, 2000). Also, PVN CRF1 receptor-expressing neurons make bidirectional connections with PVN OXY-expressing neurons, suggesting intra-PVN circuits underlying stress responses (Jiang et al., 2019). Herein, antalarmin completely eliminated morphine-induced firing of PVN OXY-expressing neurons and sociability deficits in male mice. This suggests that pharmacological disruption of the stress-responsive CRF1 receptor confers stress resilience, which per se does not require PVN OXY activity to cope with a stress-like state, leaving unaltered the expression of social behavior. On the other hand, antalarmin did not affect the activity of neurons expressing AVP, but not OXY, in male mice. Prior work suggests a minor role for AVP in stress resilience and sociability, as compared to OXY (Lukas et al., 2011; Neumann and Landgraf, 2012). Nevertheless, further studies are needed to better understand the relative contribution of PVN OXY and AVP circuits to opiate-induced sociability deficits. Finally, in female mice antalarmin affected neither morphine-induced sociability deficits nor firing of OXY/AVP- or OXY-expressing neurons, revealing a sex-specific role for the CRF1 receptor in opiate-induced activity of brain OXY systems and related social behavior.
In summary, herein we provide initial evidence of a major, sex-linked, role for the CRF1 receptor in social behavior and brain alterations induced by morphine. Indeed, disruption of CRF1 receptor function consistently eliminated morphine-induced sociability deficits and PVN neuronal firing in male, but not in female, mice. These findings suggest that inhibition of CRF1 receptor activity may relieve severe social behavior deficits commonly observed in OUD patients. Moreover, they point out to sex as a critical biological variable of studies assessing novel treatments for substance use disorders.
Materials and methods
Animals
Male and female C57BL/6J mice were bred in-house and derived from mice originally purchased from Janvier Labs (Le Genest-Saint-Isle, France). Male and female CRF1+/+, CRF1+/− and CRF1−/− mice previously generated on a mixed C57BL/6Jx129 background were bred in-house from mating CRF1+/− mice and genotype identified by PCR analysis of tail DNA (Smith et al., 1998). The colony room (22±2°C, relative humidity: 50–60%) was maintained on a 12 h light/dark cycle (lights on at 08:00). Mice were housed in groups of 2-4 in transparent polycarbonate cages (29.5 x 11.5 x 13 cm, L x W x H) containing bedding and a cotton nestlet (SAFE, Augy, France) and were 12-28 weeks old at testing. Standard laboratory food (3.3 kcal/g; SAFE, Augy, France) and water were available ad libitum. All studies were conducted in accordance with the European Communities Council Directive 2010/63/EU, were approved by the local Animal Care and Use Committee and complied with the ARRIVE Guidelines (Kilkenny et al., 2010).
Three-chamber sociability task
The three-chamber task allowed the study of the preference for an unfamiliar same-sex conspecific vs. an object and was carried out as previously reported (Piccin et al., 2022). The three-chamber apparatus was a rectangular box (60 x 40 x 20 cm, L x W x H) divided in three equal chambers and made of dark grey polypropylene. Dividing transparent Plexiglas walls had small squared doors (8 x 8 cm) that could be manually opened and closed. The central chamber was empty and each side chamber contained a round wire cage (12 cm diameter, 14 cm high, with bars spaced 1 cm apart) placed in one half-portion of the chamber. The three-chamber test was conducted during the light phase of the 12 h light/dark cycle and light intensity in the apparatus was ∼10 lux. The subject mice were handled 1 min/day during the three days preceding the three-chamber experiment. On the fourth day, C57BL/6J mice were treated with either vehicle or antalarmin (20 mg/kg) and returned to their home-cage. One hour later, they were treated with either saline or morphine (2.5 mg/kg) and immediately tested in the three-chamber task (Fig. 1A). CRF1+/+, CRF1+/− and CRF1−/− mice were just treated with either saline or morphine (0.625 mg/kg) and immediately tested in the three-chamber task (Fig. 3A). The three-chamber test consisted of three phases: pre-habituation, habituation and sociability. During the pre-habituation phase, the subject mouse was confined to the central chamber for 5 min. Then, the doors were opened and the mouse could freely explore the three chambers and the empty wire cages for 10 min (habituation phase). During the subsequent 10 min, the subject mouse could freely explore the entire apparatus with one wire cage containing an unfamiliar same-sex mouse and the other an object, i.e., a plastic bottle cap (sociability phase). The unfamiliar mice were C57BL/6J mice sex- and age-matched with the subject mice. During the three days preceding testing, the unfamiliar mice were handled 1 min/day and habituated to the wire cages for 10 min/day, with the wire cage habituation taking place in the three-chamber apparatus on the second and third day. The position (left or right side chamber) of the unfamiliar mouse was counterbalanced within each experimental group. Between each tested mouse, the apparatus was cleaned with water and the wire cages with 70% ethanol and then water. Videos were acquired and analyzed with a home-made tracking system. In particular, time (s) spent by the tested mouse in the regions of interest (ROIs, side half-chambers) containing the wire cages was taken as a measure of sociability (Fig. 1A). Indeed, our prior studies reliably demonstrated that the latter measure positively correlated with the number of nose-to-nose contacts with the unfamiliar mouse (Piccin and Contarino, 2020b). Moreover, ratio of time spent in the ROI containing the unfamiliar mouse positively correlated with the ratio of time spent with the nose in the wire cage containing the unfamiliar mouse (Piccin and Contarino, 2020b). Moreover, to control for locomotor activity, distance (m) travelled throughout the whole apparatus during the habituation and the sociability phases of the test was examined. Sociability ratio was calculated as percentage of time spent in the ROI containing the unfamiliar mouse over the total time spent in both ROIs containing the wire cages.
Brain slice preparation
C57BL/6J mice were injected with either vehicle or antalarmin (20 mg/kg) and, one hour later, with either saline or morphine (2.5 mg/kg). CRF1 receptor-deficient mice were just injected with either saline or morphine (0.625 mg/kg). Ten minutes after saline or morphine administration, mice were anesthetized by intraperitoneal (i.p.) injection of ketamine (100 mg/kg) / xylazine (10 mg/kg) until reflexes to tail- or toe-pinching were lost. Before brain removal, animals were intracardially perfused with an ice-cold bubbled (95% O2 / 5% CO2) sucrose-based saline solution containing (in mM): NaH2PO4 1.25, KCl 2.5, CaCl2 0.5, MgSO4 10, D-glucose 10, NaHCPO3 26. Brain tissue was rapidly removed and 300 μm coronal slices containing the PVN were cut using a vibroslicer (Leica VT100S, Leica Biosystems, Germany). Slices were then allowed to recover for at least 1 h at 30°C in a holding chamber filled with oxygenated (95 % O2 / 5 % CO2) artificial cerebrospinal fluid (aCSF) composed of (in mM): NaCl 126, KCl 2.5, CaCl2 2, MgSO4 2, NaH2PO4 1.25, NaHCO3 26, glucose 10 (pH 7.3, 290 mOsm).
Electrophysiology studies
Cell-attached patch-clamp recordings from PVN neurons were made at room temperature in current clamp conditions under continuous perfusion of oxygenated aCSF composed of (in mM): NaCl 126, KCl 3, CaCl2 1.6, MgSO4 1.5, NaH2PO4 1.25, NaHCO3 26, glucose 10. Throughout recordings, GABAergic and glutamatergic inputs were blocked with gabazine (1 μM) and 10μM of the NMDA and non-NMDA receptor antagonists 6,7-dinitroquinoxaline-2,3(1H,4H) dione (DNQX) and D(-)-2-amino5-phosphonopentanoic acid (AP5), respectively. Neurons were visualized with an upright Nikon Eclipse FN1 microscope (Nikon, Japan) with infrared illumination. Recording borosilicate electrodes were filled with an internal solution containing K-Gluconate 120 mM, KCl 20 mM, MgCl2 1.3 mM, EGTA 1 mM, HEPES 10 mM, CaCl2 0.1 mM, GTP 0.03 mM, cAMP 0.1 mM, leupeptine 0.01 mM, D-Mannitol 77 mM and Na 2 ATP 3 mM (pH 7.3). Moreover, biocytin 0.1% was added to the internal solution in order to post-visualize recorded neurons. Data were collected online with a Multiclamp 700B amplifier (Molecular Devices, USA) and acquired with Axograph X software (Axograph, Australia). Electrophysiology recordings were analyzed offline using the Axograph X software.
Immunohistochemistry and imaging
The phenotype of the patched and recorded cells was assessed by immunohistochemistry. After electrophysiological recording, slices were fixed with 4% paraformaldehyde overnight at 4°C. Biocytin was then revealed with FITC-Streptavidin (1/300, Vector Laboratories). OXY and AVP immunohistochemical labeling was performed at the same time using as first antibodies mouse anti-OXY monoclonal antibody (1/1000, Millipore MAB5296) and T-5048 Guinea pig anti (Arg8)-vasopressin antibody (1/1000, BMA biomedicals). Alexa fluor 488 goat anti-mouse IgG (1/500, Life technology) and Alexa fluor 647 donkey anti-guinea pig IgG (1/500, Life technology) were used as secondary antibodies. Immunostainings were acquired using a confocal Zeiss LSM900 microscope. Serial optical sections were obtained at a Z-step of 1.2 μm and imaged using an objective 10X or 20X /1.00 numerical aperture.
Drugs
Antalarmin hydrochloride (20 mg/kg; TOCRIS, Lille, France) was dissolved in acidified saline (pH ∼2.5) and injected per os (p.o.) by gavage. Morphine hydrochloride (0.625 or 2.5 mg/kg; Francopia, Gentilly, France) was dissolved in physiological saline and injected i.p. Control mice were injected p.o. or i.p. with the appropriate vehicle (acidified or physiological saline) and volume of administration was always 10 ml/kg.
Statistical analysis
Each mouse was assigned a unique identification number that was used to conduct blind testing and data analysis. To prevent strong initial preferences from biasing the three-chamber sociability results, animals exploring each ROI containing the wire cage for more than 80% (or less than 20%) of the total time spent in both ROIs during the habituation phase (10 min) were excluded from data analysis. The number of animals excluded within each experimental group is reported in Table S1A-B. For simplification and illustration purposes, we did not statistically compare the sexes in the behavior and electrophysiology studies. Thus, within each sex, the three-way repeated measures analysis of variance (ANOVA) with pre-treatment (vehicle vs. antalarmin) and treatment (saline vs. morphine) as between-subjects factors and side (mouse vs. object) or test phase (habituation vs. sociability) as a within-subject factor was used to analyze time spent in the ROIs or distance travelled during the three-chamber test by C57BL/6J mice. A three-way repeated measures ANOVA with genotype (CRF1+/+ vs. CRF1+/− vs. CRF1−/−) and treatment (saline vs. morphine) as between-subjects factors and side (mouse vs. object) or test phase (habituation vs. sociability) as a within-subject factor was used to analyze time spent in the ROIs or distance travelled during the three-chamber test by CRF1 receptor-deficient mice. The two-way ANOVA with pre-treatment (vehicle vs. antalarmin) or genotype (CRF1+/+ vs. CRF1+/− vs. CRF1−/−) and treatment (saline vs. morphine) as between-subjects factors was used to analyze sociability ratio and the firing frequency (Hz) results of the electrophysiology studies. The accepted value for significance was P<0.05. Following significant interaction effects, the Newman-Keuls post-hoc test was used for individual group comparisons. Statistical analyses were performed using the Statistica software (Version 10). Data graphs were created using GraphPad Prism and Adobe Illustrator.
Acknowledgements
The authors would like to thank Dr Philippe Ciofi (INSERM U1215) for the precious help with the oxytocin and vasopressin studies.
Funding sources
This study was supported by the Fondation pour la Recherche Médicale (Grant No. DPA20140629794 to AC and JB), the Agence Nationale de la Recherche (Grant No. ANR-21-CE37-0019-01 to AC), the University of Bordeaux and the Centre National de la Recherche Scientifique (CNRS), France. Funding sources had no further role in study design, in the collection, analysis and interpretation of data, in the writing of the report and in the decision to submit the paper for publication.
Competing interests
The authors declare no competing interest.
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