Lack of Social Support Raises Stress Vulnerability in Rats with a History of Ancestral Stress

Stress is a primary risk factor for psychiatric disorders. However, it is not fully understood why some stressed individuals are more vulnerable to psychiatric disorders than others. Here, we investigated whether multigenerational ancestral stress produces phenotypes that are sensitive to depression-like symptoms in rats. We also examined whether social isolation reveals potentially latent sensitivity to depression-like behaviours. F4 female rats born to a lineage of stressed mothers (F0-F3) received stress in adulthood while housed in pairs or alone. Social isolation during stress induced cognitive and psychomotor retardation only in rats exposed to ancestral stress. Social isolation also hampered the resilience of the hypothalamic-pituitary-adrenal axis to chronic stress and reduced hippocampal volume and brain-derived neurotrophic factor (BDNF) expression. Thus, synergy between social isolation and stress may unmask a latent history of ancestral stress, and raises vulnerability to mental health conditions. The findings support the notion that social support critically promotes stress coping and resilience.

. (A) Experimental design to induce multigenerational and adulthood stress in F4 females. Left: Animals of the parental generation (generation 0; F0) and their prenatally stressed pregnant daughters (filial generations 1-3; F1-F3) also received stress during late gestation. Right: the F4 generation that originated from a stressed maternal lineage received a stress challenge in adulthood while housed in standard paired housing conditions (MS + S-SH), socially secluded by singular housing (MS + S-SI), or received environmental enrichment with toys while being housed alone (MS + S-SI + T). (B) Stress and social isolation limit weight gain in ancestrally stressed rats. Grey-square zone indicates the 21-day stress period. Only MS + S-SI and MS + S-SI + T groups failed to gain weight during stress. A significant difference was observed between NMS-SH and MS + S-SI groups on the last day of stress exposure. Asterisks indicate significant difference between NMS + S-SI and MS+S-SI groups: *p ≤ 0.05. Error bars show ± SEM. tubes (9 cm inner diameter) of adjustable length. The tubes allowed the complete restraint of the animals while at the same time allowing them to breathe through perforated ends of the tube. The tubes maintained the animals in a standing position without compression of the body. All stress rats were stressed simultaneously in a quiet room with approximately 100 cm distance between restraint tubes. Control animals were transported to a room near the stress room but remained undisturbed in their home cages during the stress duration. All animals including controls received equal amounts of handling daily throughout the experiments.
Blood Samples and Corticosterone Assays. All rats in this experiment underwent blood sampling before and during stress in adulthood. The procedure for blood sampling was the same as previously reported by Faraji and others 28 . Blood samples were taken at three time points: two days prior to restraint stress (pre-stress), first day of stress when restraint stress was terminated (post-stress1; acute time point), and one day after the stress period was completed (day 22; post-stress2; chronic time point). Rats were placed in a restraint tube and blood samples were obtained by tail notch with a scalpel blade. Pre-stress blood was collected from all rats within the first 1-2 min of being placed in the tube to ensure circulating corticosterone (CORT) levels did not have the chance to significantly increase in response to the brief stress of the procedure. Acute and chronic time blood samples were collected using the same procedure. The same sampling procedure was applied to stress rats on the two time points while they were still in the tubes. All blood samples (0.5-0.6 mL) placed in heparinized tubes were then transferred to centrifuge tubes and plasma was obtained by centrifugation at 8000 rpm for 8 min. The plasma samples were stored at −20 °C until analyzed for CORT concentration using commercial radioimmunoassay kits (Salimetrics, UK). All samples were collected in the morning hours between 9:00 and 11:00 hours. The intra-and inter-assay coefficient of variations (CV) in the present study were 9.1% and 11.8%, respectively. No behavioural testing was performed on blood sampling days.
Behavioural Procedures: Morris Water Task (MWT). The hidden platform version of the MWT (155 cm diameter) was used to assess spatial performance 29 . Animals (N = 6-9) were tested by a one-day testing protocol (12 trials per animal) 2 days after stress in the morning (between 8:00 and 11:30 hours). Animals were taught to escape from the water (21 ± 1 °C) by climbing onto the hidden platform (12 cm diameter). Each trial began with the rat being placed in the pool at one of the four cardinal compass positions around the perimeter of the pool according to a pseudo-random sequence. The maximum duration of each swim trial was 60 s. The location of the hidden platform remained constant from trial to trial. Thus, we were able to assess trial-independent spatial learning. A no-platform probe trial was also performed two hours after the completion of the single session hidden platform testing as a measure for reference memory. The platform in the probe trail was removed from the pool and the rats were allowed to swim freely for 30 seconds. The MWT environment was divided into four quadrants in which quadrants 1, 2, 3, and 4 were labelled for NE, SE (target quadrant in the current study), SW, and NW, respectively. The percentage of time that the animals spent in each quadrant of the task was recorded. Movements of the animals including latency to find the hidden platform, swim speed and error index (swim error or corridor percent time) were recorded and analyzed by an image-computerized tracking system (HVS Image 2020, UK). The error index in the present study refers to the accuracy of an animal's swim trajectory within a 15-cm-wide corridor from the start point to the platform. Any deviation from this corridor during swimming was scored as an error 30 . Behavioural Procedures: Elevated Plus Maze (EPM). Anxiety-related behaviour was assessed under dim illumination in the EPM three days before and 2 days after restraint stress (ref. 31 with modification) in the afternoon between 14:30 and 18:30 hours. The apparatus consisted of two open and two closed arms (all 85 × 17 cm) and was elevated 93 cm above the floor. The open arms had no side or end walls, and the closed arms had side and end walls (45 cm high). The rats (N = 10-12) were placed individually in the central square facing either left or right open arm, and were allowed to explore the maze for 8 min. The experimenter left the room immediately after placing the rat on the maze. Each animal was tested only once before and after stress, and the behaviour of the animals in the maze was recorded by a camera (CCTV Auto tracking PTZ; SONY, Tokyo, Japan) and analysed by a computer tracking system (SINA Motiongraph, V.II, 2011, Tabriz, Iran) through analysis of the standard measures (time spent in the arms, time spent in the end of the open arms, time spent in the central square) of the EPM. Path length (distance traveled), path speed, stop time (absence of forward movement for at least 1 s or greater) and dispersion (the distribution of stops on the table) were also analysed. In order to minimize olfactory cues, the apparatus was cleaned with 70% alcohol after testing each animal.  35 to < 60 and > 60 s indicated by bubble diameter) and dispersion (including in-and out-cage stops), average distance between stops, and time spent in the cage by the computer tracking system (SINA Motiongraph, V.II, 2011, Tabriz, Iran). Specifically, path length and path speed were measured as an indicator of motivation level 28 . After each animal, the apparatus was cleaned with 70% alcohol.

Behavioural Procedures: Open-Field
Histological Analysis: Hippocampal Volumetry. Rats in all groups were randomly assigned to one of the histological and molecular assays due to the limited sample sizes. Two to four hours after behavioural testing, animals were euthanized as described previously 34 . To determine the hippocampal volume, a series of tissue sections (N = 5-6 per group) was stained with cresyl violet. The hippocampal volume in each rat was estimated according to the Cavalieri method 35, 36 using a set of 10-11cross-sections of the hippocampal area, starting from −1.40 mm and terminating at −6.80 mm relative to bregma. In the case of missing or damaged sections (less than 10 sections per rat) data were calculated as the average area values from preceding and following sections.

Molecular Analysis:
In Situ Hybridization. Animals (N = 3-4 per group) were euthanized with an overdose of sodium pentobarbital and decapitated at the end of the experiment to rapidly remove the brains. All in situ hybridization experiments were carried out as previously described in detail (ref. 37 with modifications) and all sections were run under identical experimental conditions. Briefly, brains were sectioned with a cryostat (15 µm) approximately from −1.40 to −4.52 mm relative to bregma. The fixed, air-dried sections were incubated overnight with two 33P-labelled 48-mer oligonucleotide probes in hybridization buffer and the excess and unbound probe was washed off. Brain sections were exposed to BioMax MR-1 X-ray films for 4 weeks. Three to four comparable tissue sections per animal and region were considered for further analysis. Levels of brain-derived neurotrophic factor (BDNF) mRNA were analyzed and masked by optical densitometry of autoradiographic films using a computerized image analysis system (MCID, Canada) and ImageJ 1.49p (NIH, USA). BDNF mRNA data in this experiment are represented as percent of NMS-SH group.
Molecular Analysis: BDNF Protein Analysis. The enzyme-linked immunosorbent assay (ELISA) was employed to quantify BDNF protein levels 37,38 . Briefly, the tissues were homogenized in 100 × (w/v) ice-cold homogenization buffer containing a protease-inhibitor cocktail and further diluted 1:9 in this buffer to a total dilution of 1000× 37 . ELISA was performed on the homogenate using the BDNF Emax Immuno Assay Systems (Promega KK, Tokyo, Japan). Two brain areas of primary interest, the frontal cortex (~3.24 mm relative to bregma) and the hippocampus (HPC; ~−3.60 mm relative to bregma) were analysed for BDNF mRNA and protein (N = 3-4 per group). Repeated measures and one-way ANOVA, and dependent and independent sample t-tests were conducted when necessary. In the present study, one-way ANOVA was used because not all groups needed for a three-way ANOVA were available. Also, post-hoc test (Tukey) was used to adjust for multiple comparisons. In all cases, means of values were compared. Data for each behavioural test were analysed by separate analysis of ANOVA with a main between-subject factor of Group. Within-subject factors were designated for each test as appropriate, for example, Trial (1)(2)(3)(4)(5)(6)(7)(8)(9)(10)(11)(12) and Quadrant (target/other quadrants) in Morris water task, Arm (open/closed arms, central square, end of open arms) for the elevated plus-maze, Stops (duration, in-or out-cage stops) for the open field table. Also, correlation coefficients were calculated to examine the correlation between plasma CORT levels, path speed in both dry-and wet-land tasks and HPC volume. Significance levels used for statistical tests were 0.05 and are denoted by one asterisk. Data are presented as means ± SEM.

Social Isolation and Stress Synergistically Impact the Stress Response. Body Weight. A compar-
ison between NMS and MS groups did not reveal a between-group effect (p = 0.063). When all groups were compared, however, repeated measures ANOVA indicated a significant main effect of Group (F 7,84 = 8.71, p = 0.041) and a significant interaction between Group and Day (p = 0.044). Compared to other groups, only MS + S-SI and MS + S-SI + T groups failed to gain weight during stress sessions (all p ≤ 0.05, post-hoc; Fig. 1B). There were no differences in body weight before stress, however (p = 0.074). Post-stress changes in body weight, on the other hand, indicated a significant main effect of Group (F 7,83 = 12.39, p = 0.044) showing all groups gained weight across 21 days except for MS + S-SI and MS + S-SI + T (all p ≤ 0.05, post-hoc). This indicates that the synergy of the adult stress and social isolation prevented body weight gain, and toy-playing experiences during stress did not alleviate the adverse outcomes of isolation housing.
Adrenal Gland Weight. In spite of an evident decrease in adrenal gland weight in MS compared to NMS animals (0.041 ± 0.011 g vs. 0.054 ± 0.01 g), no significant difference was observed between groups (p = 0.052). Two animals from NMS-SH, two animals from NMS + S-SI, one animal from MS-SI and two animals from MS + S-SI groups were excluded from this analysis due to damage to one or both adrenal glands.
Plasma CORT. Figure 2A-D illustrates circulating levels of CORT as assessed from blood samples. Seven animals in pre-stress assessment, 11 animals in post-stress 1 and 11 animals in post-stress 2 assessments in different groups were excluded from CORT analysis due to technical issues. (i) Pre-stress: Animals showed a significant overall effect of Group (F 1,94 = 10.06, p = 0.048) with the NMS group displaying higher levels of CORT than the MS group (116.29 ± 13 ng/ml vs. 77.18 ± 15 ng/ml; panel B). (ii) Post-stress1: Increased plasma CORT levels were found in most adulthood stressed groups, especially NMS + S-SH animals on the first day (acute time point) of the adulthood stress. There was a significant effect of Group for CORT levels with the NMS + S rats demonstrating higher levels than the MS + S groups (163.82 ± 14 ng/ml vs. 104.82 ± 14 ng/ml, F 1,93 = 9.33, p = 0.04; panel C).
(iii) Post-stress2: A significant main effect of Group was observed in terms of CORT levels at the post-stress 2 time point (F 7,94 = 11.68, p = 0.037) with the MS + S-SI and MS + S-SI + T groups showing higher CORT values than other groups (all p ≤ 0.05, post-hoc). Furthermore, S-SH and S-SI groups displayed a significant effect of Group (123.02 ± 11 ng/ml vs. 166.49 ± 12 ng/ml, F 1,52 = 8.13, p = 0.041) with the S-SH rats showing lower levels of CORT than S-SI rats (panel D). Also, when compared with NMS + S-SI rats, the MS + S-SI group significantly displayed increased CORT levels at the post-stress 2 time point (F 1,18 = 21.84, p = 0.03). In summary, changes in plasma CORT in the post-stress 2 phase indicated that social isolation during adulthood stress hampered the adaptive habituation response of the HPA system to chronic stress that was observed in social housing conditions. Histological Assessment. Hippocampal Volume. Isolation during adulthood stress led to smaller HPC volume in both MS + S-SI and MS + S-SI + T groups compared to other MS and NMS groups (main effect of Group: F 7,34 = 10.18, p = 0.041; Also, all p ≤ 0.05, post-hoc, Fig. 3A,B). A comparison between MS + S-SH and MS + S-SI groups indicated that socially secluded animals had lower HPC volume by 18%, and ~22% smaller HPC volume than the NMS + S-SH group. Furthermore, MS + S-SI and MS + S-SI + T rats showed approximately 20% smaller HPC volume when compared with NMS + S-SI rats. Thus, enrichment with toys during stress did not protect isolated animals against the aversive consequences of social isolation.
BDNF mRNA Expression. Although there were no changes in the frontal cortex (p = 0.34), in situ hybridization revealed that BDNF mRNA in the HPC was abundantly and differentially expressed in the DG, CA2 and CA3 but not in the CA1. A representative autoradiograph of the hippocampal BDNF mRNA expression from all experimental groups is shown in Fig. 3C). Most MS groups, especially animals subjected to adulthood stress and social isolation, showed a marked decrease in BDNF mRNA in the HPC sub-regions. A significant main effect of Group (F 7,18 = 18.51, p = 0.042) and Region (F 3,18 = 11.06, p = 0.04) but not Group by Region effect was observed in MS-SI, MS + S-SI and MS + S-SI + T animals based on prominent decrease in mRNA expression (Fig. 3D). When compared with NMS + S-SI, MS-SI and MS + S-SI + T groups, the MS + S-SI group indicated a significant decrease in mRNA expression in the DG and CA2 (main effect of region: F 3,9 = 11.37, p = 0.036; all p ≤ 0.05, post-hoc) suggesting that social isolation during stress had a noticeable impact upon mRNA expression in the

BDNF Protein Expression.
There was no significant between-group effect for BDNF protein levels in frontal cortex (p = 0.73). Also, in the HPC there was no difference between NMS (i.e. NMS-SH, NMS + S-SH and NMS + S-SI) groups despite a slightly increased level of HPC BDNF protein in NMS + S-SI (Fig. 3E). Therefore, an average of all NMS rats (205 ± 12 ng/g) was considered for baseline levels of the BDNF protein in the left and right HPC. ANOVA indicated no differences between right and left HPC in terms of BDNF proteins (p = 0.96). In all groups (except NMS + S-SI) subjected to social isolation, BDNF protein expression in the HPC was significantly decreased (168 ± 11.66 vs. 200.75 ± 11.75 ng/g; F 1,19 = 11.18, p = 0.043) when compared with animals housed in pairs (standard housing). Although adulthood stress alone did not have a significant impact on hippocampal BDNF, adulthood stress and social isolation in multigenerationally stressed animals reduced BDNF proteins to about ~18% of basal levels.

Social Isolation and Stress Impair Spatial Learning and Generate a Heightened Emotional State.
Spatial Performance in MWT. Latency and swim length are standard indicators of successful spatial navigation Here, only latency (time to find hidden platform) and speed are reported. A significant effect of Group (N = 6-9; F 7,54 = 26.11, p = 0.042) and Trial (F 11,54 = 17.91, p = 0.036) was found in terms of the latency in the MWT (Fig. 4A). Group × Trial effect was also significant (p = 0.033). Post-hoc comparison indicated that MS + S-SI and MS + S-SI + T rats spent more time (both p < 0.05) to find the hidden platform than any other group. Swim speed during the 12-trial-acquisition period showed a relatively flat speed line across 12 testing trials in all groups (Fig. 4B). The MS + S-SI rats navigated more slowly through the environment than other groups as testing proceeded. No significant difference, however, was observed between groups in terms of swim speed (p = 0.078). Analysis of spatial error via corridor percent time in the MWT (Fig. 4C,D) indicated that MS + S-SI and MS + S-SI + T rats did not directly swim to the platform (F 7,54 = 18.66; post-hoc: both p ≤ 0.05) when compared with other groups. This observation suggests inaccurate spatial navigation in multigenerationally stressed animals who experienced stress and social isolation during adulthood. A one-one way ANOVA also indicated that NMS + S-SI rats did not improve the percent time spent in the corridor when trial 1 and 12 were compared (p = 0.084). Moreover, probe trial (30-s duration, Fig. 4E,F) showed that rats in all groups displayed similar preference to spend time in the target quadrant (between 39.71-46.39%; quadrant two; SE) but MS + S-SI rats spent less time (27.98%). Thus, MS + S-SI rats arguably used a more diffuse pattern of searching, with much less spatial bias toward the former training quadrant when compared with other groups (all p ≤ 0.05, post-hoc). Examination of swim speed in the probe trial revealed no significant difference between groups.
Overall, results in the MWT indicate impaired working memory in the MS + S-SI and MS + S-SI + T rats. Dwell time in the quadrant that formerly contained the platform, also, was significantly lower for both groups relative to their controls (including NMS + S-SI) indicating an impaired reference memory. Hence, cognitive impairment in these groups became evident only after combined exposure to the two psychological adversities in adulthood.

Anxiety-related Behaviour in EPM.
Emotionality and anxiety-related behaviours were examined in the EPM (Fig. 5A-N). In all measures, MS + S-SI and MS + S-SI + T spent more time in the closed arms (  As can be seen in panel I, the distance traveled by the MS + S-SI and MS + S-SI + T groups was equally short. No significant difference was found between the groups (post-hoc: p = 0.14). Furthermore, a separate one-way ANOVA conducted for path length in NMS groups (NMS-SH, NMS + S-SH and NMS + S-SI) showed a significant effect of Group (F 2,24 = 10.49, p = 0.04) where only NMS + S-SI rats displayed shorter path length in the field when compared to NMS-SH animals (post-hoc: p ≤ 0.05; panel I). Because path length can be potentially affected by differences in path speed, both indices were considered complementary indicators of motivation in the OFT.
All groups displayed relatively constant speed (panel J) during free exploration on the table but the MS + S-SI and MS + S-SI + T groups (F 7,64 = 27.49, p = 0.041; post-hoc: both p ≤ 0.05) exhibited significantly lower speed than other groups. Also, the increased duration of stops (stop time) in MS + S-SI and MS + S-SI + T rats (F 7,64 = 18.12, p = 0.037; post-hoc: both p ≤ 0.05; panel K) indicated that adulthood stress along with social isoaltion reduced locomotor activity and exploration in the OFT, and that toy-playing experiences could not reduce the adverse motivational consequences of the loneliness during stress in multigenerationally stressed animals. Further analysis conducted with one-way ANOVA indicated that NMS + S-SI rats spent more times in stop during exploration compared to NMS-SH group (effect of Group:F 2,24 = 8.52, p = 0.043; post-hoc: p ≤ 0.05; panel K). A significant main effect of Group was found in terms of the average distance between stops (F 7,63 = 19.27, p = 0.038; post-hoc: both p ≤ 0.05; panel L) suggesting that lower speed in the MS + S-SI and MS + S-SI + T groups was also associated with fewer stops during excursion than other groups.
Stop duration measured for inside or outside the home cage on the OFT served as an additional indicator of free exploration. Again, a main effect of Group (F 7,65 = 22.91, p = 0.03; panel M) associated with significant effect of In-Out (F 1,65 = 37.16, p = 0.01) was observed. Thus, MS + S-SI and MS + S-SI + T groups spent more time inside the home cage when compared with other groups (post-hoc: both p ≤ 0.05). These data suggest that adulthood stress associated with loneliness in multigenerationally stressed rats promotes behaviours that may be implicated in the development of depression-like behaviours.
Correlation Assessment. Correlations between neurohormonal and motivational responses revealed a significant negative correlation between CORT levels in post-stress 2 and path speed in EPM (r = −0.851, p = 0.002) and OFT (r = −0.797, p = 0.010) but not MWT (r = 0.578, p = .133) only in MS + S-SI rats (N = 8-10). Thus, HPA axis hyperactivity was associated with a motivational deficit only within dry-land tasks. Furthermore, CORT levels of post-stress 2 correlated negatively with HPC volume (r = −0.721, p = 0.019) in the MS + S-SI group which suggests that high CORT values were associated with smaller hippocampal volume. No other significant correlations were found (data not shown).

Discussion
The present study provides the first account of synergistic interactions between two adverse events in female rats with a history of four generations of multigenerational stress. The major findings of this study include the following: (1) gestational prenatal stress can induce cumulative effects that remain silent across four generations and (2) generates a phenotype that is vulnerable to a depression-like state in adulthood when challenged with stress; (3) neither social isolation nor adulthood stress individually unmask the latent neuro-behavioural consequences of ancestral gestational stress in F4 rats; however (4) F4 stressed rats that were socially isolated during adulthood stress displayed dysregulation of HPA-axis activity, hippocampal atrophy and psychomotor retardation, a delayed onset of depression-relevant changes induced by synergy between two hits of stress.
The present study addressed the effects of ancestral stress in interaction with stress in later life by using the physiological measures, such as body and adrenal gland weight as well as plasma CORT level. Stress exposure across four generations did not affect body and adrenal gland weight but the CORT level: the basal plasma value in MS rats was significantly lower than in NMS rats. The blunted basal CORT along with unaffected emotionality after prenatal stress was previously reported in female rats and linked to sex-specific genetic and epigenetic regulation 40 . From a psychopathological view, multigenerational stress may lead to blunted responsiveness of the HPA axis to recurrent stress and sensitize individuals to psychiatric disturbances, thus mimicking hypocortisolism, a characteristic maladaptive neurohormonal stress response that predicts risk of post-traumatic stress disorder (PTSD) 41 .
Also, multigenerational stress may down-regulate the HPA axis activity to the level of what is commonly referred to as stress resilience when challenged with recurrent stress 42,43 . This response represents a dynamic process activated by a potentially traumatizing prolonged event 44,45 or even an active coping response 46 to ancestral recurrent adversities. Hence, our data indicate that ancestral adverse experiences enhance stress tolerance in the subsequent offspring and promote resilience across four successive generations, although HPA-axis dysregulation and/or adaptive mechanisms that might contribute to resilience are still not completely understood 47 .
When exposed to the second hit by stress in adulthood, ancestrally stressed animals showed an exacerbated response of the HPA axis that abolished resilience. Consequently, CORT levels in the MS + S-SI rats remained significantly elevated at the chronic time point relative to its values at the pre-stress level. Similar chronic glucocorticoid elevations caused by impaired HPA negative feedback have previously been linked to depression in humans 48 and depressive-like behaviours in animals 49 . By contrast, NMS or even MS rats challenged with adulthood stress but housed in pairs during stress were able to return to their pre-stress CORT values and habituate in terms of HPA axis activity 50 .
The present observations support the concept of a two-hit hypothesis 25,26 proposing that females become vulnerable to altered affective states, such as anxiety, after exposure to recurrent stress 51 . Heightened vulnerability to disease may occur through cumulative wear and tear by stress, according to the concept of allostatic load 52,53 . Body weight, on the other hand, displayed an alternative profile of adaptation; only MS + S-SI rats failed to gain weight influenced by the cumulative effects of stress and social isolation. Here, stress-induced inhibition of food intake resembles those described earlier 54,55 , and corticotropin-releasing hormone (CRH) released and neuropeptide Y (NPY) secreted by the hypothalamus during stress have been shown to impede food intake and inhibit body weight gain 56,57 .
In addition, combined exposure to stress and isolation challenges in F4 stressed rats also induced HPC atrophy and dysfunction in the absence of detectable adverse effects on the frontal cortex, although both structures are sensitive to chronic stress exposure [58][59][60] . More importantly, dysfunction of these brain regions has been reported in depression 61 . The HPC, specifically, seems the most widely investigated structure in relation to depression because it shows the highest density of corticosteroid receptors in the brain 62 and physiologically is closely connected to the inhibitory feedback in the HPA system 63,64 . Here, HPC atrophy and decreased BDNF mRNA and protein expression in ancestrally stressed rats supports the double-hit hypothesis and provides further evidence that reduced HPC volume may be a trait characteristic for depression 65 . Further quantitative BDNF analyses and evaluations of HPC neuroanatomy would be required to provide additional mechanistic links. It should be noted, however, that changes in hippocampal spatial function must not be defined merely based upon HPA-axis dysregulation or elevated plasma CORT 66, 67 even though CORT might still be causally involved in such alterations.
In addition to cognitive impairments, social isolation during adulthood stress in F4 ancestrally stressed rats triggered vulnerability to depressive-like behaviours. F4 stressed rats who were socially isolated during stress displayed motivational deficits (e.g. decreased path length and speed, and enhanced stop time 68, 69 and more avoidance behaviours 33 reflected by increased time spent in the closed arms in the EPM and inside the home cage within the OFT). These inhibitory effects on exploratory behaviours may be linked to high emotionality (anxiety and fear), fatigue and behavioural despair 70 .
The eight-group design of the present study allows dissociation of motivational and emotional changes in multigenerationally stressed animals based on single-vs. double-hit paradigms. The design confirms that only a synergy between adulthood stress and social isolation in F4 stressed rats can articulate the latent vulnerability to behavioural deficits and alter the normal profile of motivation related to depression with a sustained effect on body weight in adulthood. Maladaptive neurohormonal responses may also indicate that ancestrally stressed rats experienced high emotionality associated with the lack of social support during isolation. Therefore, the present double-hit protocol not only confirms an impaired adaptive habituation indicated by the lasting CORT elevation but also greater psychomotor inhibition shown by the failure to gain weight in ancestrally stressed rats.
The observation that social support mitigates the adverse consequences of stress is in agreement with earlier findings. A recent study by Seetharaman and others 71 indicated that daily exposure to a social environment reduces the risk of PTSD-like effects in rats. The authors suggested that social stimulation may reduce traumatic memories and therefore lead to reduced fear-related behaviour 71 . In addition, social support is particularly effective in reducing PTSD risk, chronic anxiety and stress 72 while the lack thereof is associated with greater stress response and PTSD risk 73,74 . In addition, interventions that provide social support can reduce perceived stress during pregnancy 75 , improve early brain development 76 and mental and cognitive health 77 . The present experimental data not only support these findings, but suggest that social stability and support may alleviate the transgenerational transmission of stress and thus potentially improve mental health outcomes.
The present results also linked the effect of stress to structural changes and synaptic connectivity in association regions of the brain (e.g. HPC) and animal behaviour, although the effects of multigenerational stress in brain circuits are not well understood 78 . We believe repeated functional assessment using optogenetic 79 and imaging tools [80][81][82] combined with animal behaviour is ideally suited to monitor in real time the process by which multigenerational stress changes the structure and function of different brain circuits.