DSCR9 gene simultaneous expression in placental, testicular and renal tissues from baboon (papio hamadryas)

Background In 2002 Takamatsu and co-workers described the human DSCR9 gene and observed that it was transcriptionally active in human testicular tissue, but no protein was identified as a product of this transcript. Similar results were obtained in chimpanzee tissue. This gene has not been detected in species other than primates, suggesting that DSCR9 is exclusively found in these mammals. Results We report evidence of DSCR9 expression in placenta, testis and kidney of baboon (Papio hamadryas). We used primers specific for DSCR9 to amplify transcripts through reverse transcription (RT) coupled to polymerase chain reaction (PCR). Furthermore, PCR was used to amplify the complete DSCR9 gene from genomic DNA from three baboons. We amplified and sequenced five overlapping segments that were assembled into the 3284 bp baboon DSCR9 gene, including the putative promoter and the entire transcriptional unit (5'-UTR, CDS and 3'-UTR). Conclusions The baboon DSCR9 gene is highly similar to the human counterpart. The isolated transcripts from baboon tissues (placenta, testis and kidney) of three different baboons correspond to the human orthologous gene.


Background
Down syndrome (DS) or trisomy 21 is the most common chromosome disorder affecting newborns and the most frequent and recognized cause of mental retardation in Homo sapiens (Hosa) [1]. The incidence of this syndrome is about 1 in 700 newborns [2]. Chromosome 21 is the smallest of human autosomal chromosomes, and an extra copy or additional segment of this chromosome causes DS [3]. The chromosomal region responsible for this pathology has been described [4] and named Down Syndrome Critical Region (DSCR) [5,6]. By comparing the genomic DSCR sequence in humans with that of other species, it was shown that it is highly conserved in great apes [6] and similar trisomies have been described in these non human primates [7,8]. In humans, ten potential genes have been identified in the DSCR, two of which (DSCR9 and DSCR10) are exclusive of primates [9]. In man, DSCR9 gene transcription, but not proteins, were evidenced in testicle; this was also demonstrated in chimpanzee [9]. The aim of this study was to identify the chromosome segment from which the DSCR9 gene´s transcripts originated.
We amplified five segments from the baboon genome using primers designed to render overlapping amplicons. Using this strategy we were able to assemble the complete DSCR9 gene of the species. The isolated genomic segment includes the putative promoter and the complete transcriptional unit. Using reverse transcription (RT) coupled to polymerase chain reaction (PCR), we have gathered evidenced of the expression of the DSCR9 gene in baboon's placenta, testicles, and kidney, an of its lack of detectable expression in heart, omental fat, skeletal muscle, pancreas, mononuclear cells, liver, and hypothalamus. The identified transcripts of these tissues in three different individual were identical and correspond to the isolated DSCR9 baboon gene.

Animal specimens
Animal procedures were performed according to ethical guidelines and reviewed by the Institutional Animal Care and Use Committee of the Texas Biomedical Research Institute (TBRI). Animals were maintained at the Southwest National Primate Research Center in San Antonio, Texas at TBRI. All the animals shared the same diet and environmental conditions before and during pregnancy. All baboons are gang-housed and fed ad libitum on a standard low-fat chow diet (Harlan Tecklad 15% Monkey Diet, 8715).

Biological samples
Different tissues from tree male baboons (testis, kidney, heart, omental fat, skeletal muscle, pancreas, mononuclear cells, liver, and hypothalamus) and from tree female baboons (ovary and placenta) were collected in programmed necropsies, under fasting conditions. Placental tissues were collected by caesarean section at the time of birth [at the term period of gestation for this species (136 to 139 days)]. All tissues were stored in liquid nitrogen immediately after collection until needed.

Nucleic acid isolation from placental tissue
Genomic DNA and total RNA were isolated from each tissue using TRIZOL reagent; procedures were performed according to the manufacturer's instructions (Invitrogen, Carlsbad, CA). RNA samples were treated with DNase I (Invitrogen) for 10 min at 37°C to remove traces of genomic DNA, genomic DNA was treated with RNase I (Invitrogen) for 30 min at 37°C to remove traces of RNA. RNA and DNA quality and integrity were assessed by standard spectrophotometric and electrophoretic methods, respectively.

Reverse transcription
RT reactions were carried-out with 1 μg of total RNA using random primers and a High-capacity cDNA Reverse Transcription kit, following manufacturer's instructions (Applied Biosystems, Foster City, CA).

Primer design
To amplify baboon DSCR9 gene and transcript, primers were designed based on highly conserved primate DSCR9 sequences previously reported [great apes and old world monkeys (OWMs)] and using the online primer-3 tool [10]. Primers (see Table 1) were designed to amplify overlapping target template sequences in order to isolate the complete DSCR9 gene (in concordance with human gene structure).

PCR amplification
To amplify DSCR9 gene from genomic DNA five primer sets were used in separate PCR reactions (Table 1). Each PCR reaction was performed in 50 μl reaction containing 10 pM of each primer, 200 ng of genomic DNA and 2X PCR master mix (Qiagen, Valencia, CA). To amplify DSCR9-related transcript, a primers set (see Table 1) was used with 10 pM of each primer and 5 μl of RT reaction from each tissue. PCR amplification programs are described in Table 1. Universal 18 s ribosomal gene primers were used in RT-PCR as positive control. (Ambion, Austin, TX). PCR amplifications were confirmed by electrophoresis in agarose gel (1%) run in TAE X1 buffer, stained with etidium bromide and visualized under UV light.

Molecular cloning and sequencing
PCR products were cloned using the TOPOXL cloning system with the pCR-XL-TOPO 3.5 kb vector (Invitrogen). Ligation reactions were transformed into electrocompetent Top 10 Escherichia coli bacterium according to the manufacturer's instructions (Invitrogen). Cloning products were sequenced in an ABI PRISM 3100 Genetic Analyzer (Applied Biosystems) using universal M13 primers, and Big Dye terminator reagent (Applied Biosystems). Novel sequence has been deposited in the GenBank database (Accession number: JF775469).

Sequence analysis
Electropherograms were analyzed using GeneStudio Pro software (GeneStudio, Inc., Suwanee, GA). Procedures were carried out in three clones for each amplicon to exclude artifacts. DNA sequences from DSCR9-related transcripts were used to determine the amino acid sequence using the Transeq online program [11] and were subsequently aligned using the ClustalW program [12] and Vista tools [13]. The alignments were performed using peptide sequences extracted from GenBank [14] by homology search.

Baboon DCSR9 gene isolation
Baboon genomic DSCR9 gene was isolated by PCR in five overlapping segments (see Figure 1), which were cloned and sequenced. The assembled sequenced gene was submitted with the BLAST tool of NCBI to the GenBank and match was confirmed with the human DSCR9 gene (data not shown).

DSCR9 gene of papio hamadryas
The assembled baboon DSCR9 gene lacks a TATA box, conventional Kozak sequence [15,16], introns, and polyadenylation signal. The baboon DSCR9 gene has a structure similar to its human counterpart ( Figure 2) but with

DSCR9 gene putative promoter analysis
Based on the structure of the DSCR9 human gene, we performed the amplification of an upstream region of the transcriptional unit, which we proposed as the putative promoter. The obtained sequence was compared with its counterpart in Hosa [9], which was 93% identical (see Figure 3). Additional experiments of transcriptional activity are required to validate the promoter activity of this DNA segment.

Papio hamadryas DSCR9 transcript detection
In order to determine DSCR9 gene expression in baboon, total RNA was extracted from testis, kidney, cardiac, omental fat, skeletal muscle, pancreas, mononuclear cells, liver, and hypothalamus, placenta and ovary tissues. Total RNA was used for cDNA synthesis by RT. For DSCR9 transcript isolation an oligo set was designed consisting of a forward consensus primer (DSCR9-rnaF) hybridizing at 148 bases upstream from the translation initiation codon (AUG) and a reverse primer (DSCR9-rnaR) annealing 36 bases after the termination codon (UGA) (positions according to Hosa DSCR9 mRNA [9]). We detected an amplified product in three different tissues: placental, testis and kidney. A single band was amplified in each case. The size of the amplified product (Paha: 726 b) was larger than expected, according to the human sequence (Hosa: 673 b). We used amplification of ribosomal RNA 18 s as positive control for each tissue. Negative and positive controls gave the expected results. Expression in heart, omental fat, skeletal muscle, pancreas, mononuclear cells, liver, and hypothalamus was discarded, at least to the sensitivity levels of the used RT-PCR techniques. The baboon DSCR9 gene sequence, which is also that of its mRNA since it is an intronless gene, was compared with its Hosa counterpart and found to be 90% identical. This value decreases to 89% if just the CDS of both genes are compared. A single thymine nucleotide insertion (underlined in black) results in a premature stop codon (showed in a box), which is predicted to decrease the polypeptide length to 50 aa (see Figure 2). Consequently, from this point on both conceptually translated proteins lose their similarity.

Discussion
The expression of DSCR9 gene evidenced in baboon's testicular, kidney and placental tissues coincides with previous reports of expression in humans in the former tissue, but differs in that of the later two organs. The sequences of DSCR9 gene transcripts in all baboon tissues were identical and without evidence of alternative splicing, unlike those reported for human in which eight different mRNA  species have been described (see Table 2). Currently, the predicted DSCR9 protein has not been detected and thus the function of this gene remains unknown. It is hypothesized that allelic variants of the DSCR9 gene may influence the accumulation of connective tissue of the iris resulting in the phenotype of a different eye color [10]. Probably the DSCR9 gene is expressed constitutively in the iris and/or acts in a regulatory manner through RNA interference and/or modifies the expression of other genes in the tissue that is associated with a specific phenotype.

Conclusion
In our study we found a homologous region to the human DSCR9 gene in the Papio hamadryas genome. We provide evidence of the expression of DSCR9 gene in baboon's testicular, kidney and placental tissues and of lack of expression in heart, omental fat, skeletal muscle, pancreas, mononuclear cells, liver, and hypothalamus. The segments that compose the transcript unit were assigned based on the strategy described previously by Takamatsu, et al. [9]. Experiments like RNA-RACE are necessary to found 5'-CAP element and designate the length of the 5'-UTR (size in nucleotides). We proposed our gene elements´nomenclature according to the gene annotation made by Takamatsu et al. [9]. According to our findings, the predicted baboon 5´-UTR has a second ATG sequence that initiates a putative ORF of only three amino acids in length. Then, we agreed with the start codon proposed by Takamatsu et al. [9]. The function of this gene remains unknown, but at least in baboon seems to be dispensable since its corresponding mRNA has a single nucleotide insertion that results in a premature termination of protein. Further studies on the function of this protein in human and other primates are required to understand its role and possible association with the DS phenotype.

Competing interests
The authors do not have any potential or actual personal, political, or financial interest in the material, information, or techniques described in this paper. Callithrix jacchus SRR000079** SRR000079** * = Core subset of nucleotide sequence records, ** = SRA, *** = EST of GenBank at the NCBI.