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The ATP-binding cassette transporter ABCC6 gene is located on chromosome 16 between its two pseudogenes (ABCC6P1 and ABCC6P2). Previously, we have shown that ABCC6P1 is transcribed and affects ABCC6 at the transcriptional level. In this study we aimed to determine copy number variations of ABCC6, ABCC6P1 and ABCC6P2 in different populations. Moreover, we sought to study the transcription pattern of ABCC6 and ABCC6 pseudogenes in 39 different human tissues.
Genomic DNA from healthy individuals from five populations, Chinese (n=24), Middle East (n=20), Mexicans (n=24), Caucasians (n=50) and Africans (n=24), were examined for copy number variations of ABCC6 and its pseudogenes by pyrosequencing and quantitative PCR. Copy number variation of ABCC6 was very rare (2/142; 1.4%). However, one or three copies of ABCC6P1 were relatively common (3% and 8%, respectively). Only one person had a single copy of ABCC6P2 while none had three copies. In Chinese, deletions or duplications of ABCC6P1 were more frequent than in any other population (9/24; 37.5%). The transcription pattern of ABCC6P2 was highly similar to ABCC6 and ABCC6P1, with highest transcription in liver and kidney. Interestingly, the total transcription level of pseudogenes, ABCC6P1+ABCC6P2, was higher than ABCC6 in most tissues, including liver and kidney.
Copy number variations of the ABCC6 pseudogenes are quite common, especially in populations of Chinese ancestry. The expression pattern of ABCC6P2 in 39 human tissues was highly similar to that of ABCC6 and ABCC6P1 suggesting similar regulatory mechanisms for ABCC6 and its pseudogenes.
The ATP-binding cassette transporter ABCC6 belongs to a large family of membrane proteins (ABC transporters) that are a highly conserved and present in all organisms from bacteria to man [1,2]. The ABCC6 gene (Entrez Gene ID 368) is located on the short arm of chromosome 16 along with two shorter, almost identical (> 99% sequence identity), pseudogenes; ABCC6P1 (Entrez Gene ID 653190) and ABCC6P2 (Entrez Gene ID 730013) (Figure (Figure1)1) . Pseudogenes are generally defined as non-functional genes, meaning that they usually do not produce a transcript or a functional protein [4,5]. Transcription of ABCC6 pseudogenes have been described [3,6,7], and recently we found strong evidence for a regulatory interdependency between ABCC6 and its pseudogene ABCC6P1.
Mutations and deletions in ABCC6 are known to cause the rare (prevalence between 1:25,000 and 1:100,000), autosomal recessive disease pseudoxanthoma elasticum (PXE, OMIM 264800), a metabolic disorder characterized by ectopic mineralization of soft connective tissues [8,9]. ABCC6 is located on chromosome 16, a known hotspot of chromosomal instability, showing several genomic duplications and deletions (generally called copy number variations) [10,11]. We therefore hypothesized that ABCC6 pseudogenes would be liable to chromosomal rearrangements and thereby subject to copy number variations. Having less or more copies of ABCC6 pseudogenes is likely to influence the expression level of these pseudogenes, and thus, may have an impact on the parent gene ABCC6, including the genetic message, the protein level and the function of the protein.
Estimation of copy number variations and transcription of pseudogenes is generally difficult because of the high sequence similarity between pseudogenes and their parent genes. However, pyrosequencing has recently shown to be a helpful tool to differentiate between highly similar genes by only one nucleotide difference . Therefore, principally by the use of pyrosequencing, the aim of this study was to determine copy number variations of ABCC6ABCC6P1 and ABCC6P2. Moreover, we sought to study the mRNA transcription pattern of ABCC6ABCC6P1 and ABCC6P2 in 39 different human tissues.
Copy number variation of ABCC6 was very rare (2/142; 1.4%) (Table (Table1)1) in healthy individuals. No individuals had deletions of ABCC6. Deviation in copy number was more frequent for ABCC6 pseudogenes. In Chinese, deletions or duplications of ABCC6P1 were more frequent than in any other population (9/24; 37.5%). Furthermore, in the total population (n=142), one or three copies of ABCC6P1 was relatively common (3% and 8%, respectively). Only one person had one copy of ABCC6P2 while none had three copies. In Africans, however, no copy number variation was found for ABCC6 pseudogenes. All the members of two Centre d’Etude du Polymorphisme Humain (CEPH) pedigrees had two copies of ABCC6, ABCC6P1 and ABCC6P2 (data not shown). As copy number variation was analyzed in short specific regions of ABCC6 and ABCC6 pseudogenes, small deletions/insertions in other regions of these genes cannot be excluded.
ABCC6 and ABCC6 pseudogene expression profiling was performed in various human tissues (not corresponding to individuals analyzed for copy number variations). The transcription pattern of ABCC6P2 was highly similar to ABCC6 and ABCC6P1, with highest transcription in liver and kidney (Figure (Figure22 A-C). Interestingly, the total mRNA level of ABCC6 pseudogenes, ABCC6P1+ABCC6P2, was higher than ABCC6 mRNA levels in most tissues, including liver and kidney (Figure (Figure22 D). However, it should be noted that in tissues with low ABCC6 mRNA levels, differences in expression between ABCC6 and its pseudogenes may result from stochastic effects during the PCR.
In this study, we found copy number variation of ABCC6 pseudogenes to be frequent, especially in populations of Chinese ancestry. However, as expected in healthy populations, no individuals had deletions of ABCC6. ABCC6 and its pseudogenes, with their high sequence identity (>99%), represent a low copy repeat (LCR). LCRs are paralogue segments of usually >10kb with >97% sequence identity and can act as substrates for nonallelic homologous recombination which may lead to deletion, duplication or inversion of the intervening sequence [13,14]. Phylogenetic trees on human and chimpanzee sequences show that ABCC6 pseudogenes have occurred independently several times in these species, which further demonstrate the high mobility of these genes . Our results confirm the hypothesis that ABCC6 pseudogenes would be liable to genomic instability and thereby copy number variations.
Six percent of Caucasians are expected to have three copies of ABCC6P1 (Table (Table1).1). However, none of the 35 members of two 3-generation-pedigrees (CEPH pedigrees) had deviation from the normal copy of two of ABCC6 or ABCC6 pseudogenes, indicating a Mendelian transmission of these copy numbers and that de novo deletion/duplication of pseudogenes do not arise frequently.
ABCC6 and its pseudogenes share highly similar proximal promoter sequences (> 98.5% sequence identity) . Furthermore, the hepatocyte nuclear factor 4α (HNF4α) binding site located at −166/-154 of the ABCC6 promoter, which is crucial for tissue-specific expression pattern of ABCC6[16,17], is also present in the ABCC6P1 and ABCC6P2 promoters. Thus, the finding of similar expression pattern for ABCC6 and both pseudogenes in human tissues strongly imply similar regulatory mechanisms for ABCC6 and its pseudogenes. On the other hand, these results also suggest that both ABCC6- and ABCC6 pseudogene transcripts have similar half-lives, which is surprising since they do not share the same mRNA 3’-ends. Pseudogenes were for a long time assumed to be “junk DNA”. However, recent studies have shown that many pseudogenes are functionally active and that they may influence their parent gene [7,18-23], and potential mechanisms of pseudogene function have been suggested. Copy number variation in pseudogenes has previously also been identified for the Neutrophil cytosolic factor 1 (NCF1) pseudogenes [24-26]. NCF1 is a component of NADPH oxidase and having fewer or more copies of NCF1 pseudogenes seem to influence the production of reactive oxygen intermediates [24,26]. It would therefore be interesting to investigate whether different copy numbers of ABCC6 pseudogenes also influences the expression of the ABCC6 gene. Unfortunately, the expression of ABCC6ABCC6P1 and ABCC6P2 in various human lymphoblastoid cell lines with one, two or three copies of ABCC6P1, which could be used for these studies, was too low to be detected by reverse transcription - quantitative real-time PCR (RT-qPCR) or pyrosequencing (data not shown).
Genomic DNA from the National Institute of General Medical Science (NIGMS) Human Variation Panels was purchased from the Coriell Cell Repositories (Camden, USA): The Caucasian Panel (n=50); The Han People of Los Angeles Panel (n=24); The Middle Eastern Panel, version 1 and 2, (n=20); The Mexican-American Community of Los Angeles Panel (n=24), The African-American Panel (n=24) and two pedigrees (CEPH/Utah Pedigree 1331 and CEPH/Amish Pedigree 884). High quality RNA samples of the Human Total Master panel II and the Human Adult Normal Tissue Total RNA (39 tissues in total) were purchased from Clontech (Mountain View, USA) and BioCat Gmbh (Heidelberg, Germany) respectively.
For absolute copy number determination of ABCC6, the TaqMan® Copy Number Assay was used targeting ABCC6 specifically in intron 11 (Hs03952142_cn; Applied Biosystems, Foster City, USA). Rnase P, which is known to be present in two copies in the human genome, was used as endogenous reference gene (TaqMan® Copy Number Reference Assay Rnase P, Applied Biosystems). The ABCC6 assay (labeled with FAM), the RnaseP assay (labeled with VIC), sample DNA and 2xTaqMan Universal PCR Master Mix was combined in 20μl reactions and ran in quadruplicate on a 7900HT Fast Real-Time PCR System using standard conditions (Applied Biosystem). The absolute copy number of ABCC6 was thereby calculated using CopyCaller™Software v1.0 (Applied Biosystems).
For pyrosequencing, two sets of PCR primers were designed to amplify ABCC6, ABCC6P1 and ABCC6P2. The first set of primers targeted intron 7 of ABCC6 and ABCC6P1 only, while the other set of primers targeted exon 2 of all three genes (Table (Table22 and Figure Figure1).1). The genes were amplified from ~100ng of genomic DNA in 25 μL reactions using 1 x PyroMark PCR Master Mix, 1 x CoralLoad Concentrate (Qiagen, Venlo, The Netherlands) and 0.2μM primers. Cycling conditions were an initial enzyme activation step at 95°C for 15min and 45cycles of 94°C for 30s, 60°C for 30s, and 72°C for 30s, and a final extension cycle of 72°C for 10min. Twenty micro liter of PCR products were added to 40 μL Binding Buffer (Qiagen), 2 μL streptavidin sepharose high-performance beads (GE Healthcare, Little Chalfont, United Kingdom) and 18 μL water and stirred for 5–10min at 1400rpm on a mixer. Single stranded biotinylated templates were isolated using PyroMark Vacuum Prep WorkStation (Qiagen) and dispensed onto PyroMarkQ24 plate containing 25 μL of 0.3μM sequencing primer and Annealing Buffer (Qiagen). The plates were incubated for 2min at 80°C and subsequently cooled at room temperature for at least 5min. Sequencing was performed using a PyroMark Q24 instrument with PyroGold reagents (Qiagen). In the sequencing reaction, one and one nucleotide is added at the time, and peak heights are propotional to the amount of nucleotide molecules incorporated. Therefore, relative copy numbers were calculated using ratios of pyrogram peak heights: ABCC6/(ABCC6+ABCC6P1)=C5/C8 (C5 and C8 being the peak heights at dispensation 5 and 8, respectively for assay #1) and ABCC6P2/(ABCC6+ABCC6P1+ABCC6P2)=T8/T6 (T6 and T8 being the peak heights at dispensation 6 and 8, respectively for assay # 2, note; reverse sequencing) (Table (Table22).
The absolute copy number for each allele (ABCC6, ABCC6P1 and ABCC6P2) was finally deduced from the TaqMan® Copy Number Assay and the two pyrosequencing assays.
cDNA was synthesized from total RNA from 39 tissues (1μg) by reverse-transcription using Omniscript RT kit (Qiagen) in the presence of oligo-dT and random hexamer primers (Applied Biosystems) in 20 μL reactions.
Previously, the mRNA expression pattern of ABCC6 and ABCC6P1 in 20 different tissues was described by our group . In this study, we determined the mRNA expression pattern of ABCC6 and ABCC6P1 in a total of 39 tissues by RT-qPCR on a 7900HT Fast Real-Time PCR System (Applied Biosystems). Five of twelve reference genes were estimated by geNorm  to give the most reliable normalization factors (see  for assay IDs): GAPDH=PGK1>SDHA>CTBP1>GOLGA1 . The expression of ABCC6 and ABCC6P1 was normalized to these factors for each tissue.
Due to methodological issues, the mRNA expression pattern of ABCC6P2 was not investigated in our previous study . In this study, the relative mRNA expression pattern of ABCC6P2 was analyzed by pyrosequencing. Primers for mRNA expression were designed to amplify ABCC6ABCC6P1 and ABCC6P2 expressed genes (Table (Table2).2). The relative transcription of ABCC6P2 to ABCC6 and ABCC6P1 in the same 39 tissues was quantified using the same equation as above: ABCC6P2/(ABCC6+ABCC6P1+ABCC6P2)=T8/T6; Assay #3, Table Table2),2), and by using the expressional data (RT-qPCR) of ABCC6 and ABCC6P1. All PCR samples were run in parallels. No parallels varied more than 0.5 quantification cycles in qPCR experiments or 0.1 in pyrosequencing peak height ratios.
The data set supporting the results of this article are included within the article in Additional file 1 Table S1.
The authors declare that they have no competing interests.
MKK, AP and JPB participated in the study design. MKK, CS and RMG carried out the experimental work. MKK and CS did the interpretation of data. MKK drafted the manuscript with assistance from CS and AP. All authors read and approved the final manuscript.
Copy numbers of ABCC6, ABCC6P1 and ABCC6P2.
This project has been financed with aid from the South-Eastern Norway Regional Health Authority and grant from the Clinic of Diagnostics and Intervention, Oslo university hospital, Oslo, Norway.