Sex-specific cortical, hippocampal and thalamic whole genome transcriptome data from controls and a G72 schizophrenia mouse model

Objectives The G72 mouse model of schizophrenia represents a well-known model that was generated to meet the main translational criteria of isomorphism, homology and predictability of schizophrenia to a maximum extent. In order to get a more detailed view of the complex etiopathogenesis of schizophrenia, whole genome transcriptome studies turn out to be indispensable. Here we carried out microarray data collection based on RNA extracted from the retrosplenial cortex, hippocampus and thalamus of G72 transgenic and wild-type control mice. Experimental animals were age-matched and importantly, both sexes were considered separately. Data description The isolated RNA from all three brain regions was purified, quantified und quality controlled before initiation of the hybridization procedure with SurePrint G3 Mouse Gene Expression v2 8  ×  60 K microarrays. Following immunofluorescent measurement und preprocessing of image data, raw transcriptome data from G72 mice and control animals were extracted and uploaded in a public database. Our data allow insight into significant alterations in gene transcript levels in G72 mice and enable the reader/user to perform further complex analyses to identify potential age-, sex- and brain-region-specific alterations in transcription profiles and related pathways. The latter could facilitate biomarker identification and drug research and development in schizophrenia research.

Sex-specific cortical, hippocampal and thalamic whole genome transcriptome data from controls and a G72 schizophrenia mouse model Objective G72/G30 is a primate specific gene that is localized on human chromosome 13q and turned out to be a susceptibility locus for major psychiatric disorders such as schizophrenia and bipolar disorder [1][2][3].The dominant gene product of this locus is the largest G72 splice variant, i.e., LG72 protein (here referred to as G72 protein).Notably, the function of the G72 protein in neuropsychiatry remains obscure [4].Interestingly, increased G72 protein levels were observed in the serum and CNS of schizophrenic patients [5,6].In order to investigate the functional implications of the G72 protein in vivo, a humanized transgenic mouse model carrying the G72/G30 locus has been generated that expresses the G72 protein [7].G72 transgenic mice serve as a schizophrenia model as they display characteristic symptoms, such as motor coordination deficits, altered sensorimotor gating and olfactory discrimination, increased compulsive behavior and spatial memory impairment [7,8].
Previous complementary proteomics studies from the cerebellum of G72 mice revealed altered protein expression in mitochondria-associated, myelin-and oxidative stress-related processes in G72 compared to control mice [8][9][10][11].Recently, Filiou et al. (2022) performed multi-omics approaches, i.e., quantitative proteomics and metabolomics, from the hippocampus of male, eight weeks old G72 vs. control mice [10].However, we are still lacking detailed information about both sex-and brain-region specific differences in transcriptome profiles from schizophrenia mouse models such as G72.To fill this essential gap, we carried out microarray analysis of RNA from the retrosplenial (RS) cortex, hippocampus and thalamus of both female and male G72 mice.It has been shown in the past that the RS cortex is essential for gating information to the medial temporal lobe and displays aberrant connectivity with neuronal networks associated with memory formation and ecphoria, i.e., the limbic system/hippocampal formation in schizophrenia patients [12].In addition, enhanced neuronal connectivity of the RS cortex with the left superior temporal gyrus was observed in patients with more positive symptoms, e.g.hallucinations [12].Impaired function of the RS cortex was also related to verbal memory deficits commonly seen in schizophrenia patients [13].These and other findings suggest that the RS cortex is of central importance in schizophrenia symptomatology [12,14].The hippocampus as a memory consolidation and formation system has been related to schizophrenia for long.The etiopathological evolution of schizophrenia via the premorbid, prodromal to syndromal psychotic stages was shown to initiate with dysregulation of glutamate transmission in the CA1 area, further progressing to other hippocampal regions and cortical areas as well [15,16].The thalamus as part of the thalamocorticalcorticothalamic circuitry serves as another important structure in schizophrenia.It's critical for the transmission and processing of external information and thereby modulates essential tasks such as wakefulness, sleep and memory.It was shown in both animal models and humans that there are thalamic connectivity deficits in psychiatric disorders, including schizophrenia [17].There is also evidence of altered thalamic microstructure, e.g., in the mediodorsal nucleus, thalamo-prefrontal and thalamo-somatosensory/parietal connectivity [17].Multiple studies have proposed an association between psychosis spectrum disorders and thalamic network dysrhythmia and/or dysconnectivity [18,19].Our microarray data from these three highly relevant brain regions allow for further characterization of differentially expressed intersectional and signature genes of the individual subgroups, gene ontology and pathway analysis and biophysical studies [20,21] which are of relevance for future translational studies.

Experimental animals
G72 transgenic mice carrying the G72/G30 locus and wild-type (WT) mice with a CD1 background were kindly provided by the Institute of Molecular Psychiatry (Life & Brain, Bonn, Germany).Details on breeding and genetics of G72 mice have been described in detail before [7,8].In total, eight WT control animals (four ♂, age: 23.14 ± 0.00 wks; four ♀, age: 23.46 ± 0.11 wks) and eight G72 transgenic mice (four ♂, age: 23.14 ± 0.00 wks; four ♀, age: 23.14 ± 0.00 wks) were used for dissection of hippocampus, RS cortex and thalamus for subsequent transcriptome analysis.

Genotyping -DNA preparation from tail biopsies
Every experimental animal was genotyped twice using DNA isolated from tail biopsies.DNA preparation was carried out using peqGOLD DNA Mini Kit (PEQLAB Biotechnologie GmbH, Germany) according to the manufacturer's instructions.The isolated genomic DNA was stored at + 4 °C until further use.

Hippocampus, RS cortex and thalamus preparation and tissue storage
Experimental animals were anaesthetized using i.p. injection of ketamine (100 mg/kg) / xylazine (10 mg/ kg) and immediately decapitated.The brain was removed and placed in a clean RNase-free petri-dish filled with pure RNAlater reagent (Qiagen GmbH, Germany).The RS cortex, hippocampus and thalamus were bluntly dissected and immediately placed in 2 ml RNase free reaction tubes, snap frozen in liquid nitrogen and stored at -80 °C until RNA preparation.This instantaneous and fast processing was performed to eliminate potential effects of anaesthesia on early gene regulation.

Retrosplenial cortex, hippocampal and thalamic RNA isolation
Total RNA from the individual brain regions was extracted using RNeasy Lipid Tissue Mini Kit (Qiagen GmbH, Germany) according to the manufacturer's protocol.Quantity and quality of the RNA was evaluated using NanoDrop ND-1000 (ThermoFisher Scientific Inc., USA).

Acquisition of transcriptome data and raw data extraction
Transcriptome data were acquired using the One-Color Microarray-Based Gene Expression system (Agilent Technologies Germany GmbH & Co. KG, Germany).In specific, the SurePrint G3 Mouse Gene Expression v2 8 × 60 K Microarray Kit (Agilent Technologies Germany GmbH & Co. KG, Germany) was used for RS cortex, hippocampal and thalamic tissue.All procedures were carried out according to the manufacturer's instructions.
Raw data are based on fluorescence scanning using the Agilent SureScan Microarray Scanner and raw microarray image file processing using the Feature Extraction Software (both from Agilent Technologies Germany GmbH & Co. KG, Germany).Using GeneSpring Software (Agilent Technologies Germany GmbH & Co. KG, Germany), all information about probe names, fold changes, etc. were extracted and exported into txt.-andcsv.-files to allow usage in other transcriptome analysis software in case GeneSpring software is not used and/or not available.These raw data represent unfiltered, non pre-analyzed data.
The individual subgroups and related data are characterized in Table 1.

Limitations
This transcriptome data collection from the RS cortex, hippocampus and thalamus of ∼ 6 months old G72 and control mice was carried out using a microarray approach.Following scientific and organizational aspects, resource considerations, and power calculations, this turned out to be a feasible approach for us.We are aware that RNAseq is also a very good alternative strategy to characterize transcriptional alterations in the G72 schizophrenia mouse line.
The G72 mouse model is a unique schizophrenia model to characterize the impact of the G72 protein in neuropsychiatry [7,8].This may limit its generalizability compared to other schizophrenia models as regards isomorphism, homology and predictability representing the major translational categories in biomedicine.As for other diseases, numerous schizophrenia mouse models have been generated and none of these models can claim to mimic the etiopathogenesis, symptomatology and drug delivery characteristics of the human disease equivalent to a 100% [22][23][24].Given these observations, searching a schizophrenia model with common trans-line and trans-species transcriptional profiles is highly challenging.We have thus decided to use the humanized transgenic mouse model G72 carrying the G72/G30 locus which has received much attention in literature, and which can provide novel insight into the crucial role of G72 protein in the etiopathogenesis of schizophrenia.
A unique feature of our data is related to their sexand brain region-related specificity.Clearly, this results in a high number of experimental subgroups (twelve in total) and microarrays to be used.Note that we focused on animals of "older" age (i.e., 23 wks) in this data collection as stereotypic behavior, characterized by repetitive and unintentional movements typically appears in progressed disease stages [25][26][27][28].To get an impression of temporal effects on G72 transcriptome profiles, additional studies with G72 and control animals of different ages are necessary.