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The Journal of Clinical Investigation logoLink to The Journal of Clinical Investigation
. 2012 Jun 18;122(7):2439–2443. doi: 10.1172/JCI63597

Exome sequencing identifies GATA1 mutations resulting in Diamond-Blackfan anemia

Vijay G Sankaran 1,2,3,4, Roxanne Ghazvinian 5, Ron Do 1, Prathapan Thiru 2, Jo-Anne Vergilio 6, Alan H Beggs 4,5, Colin A Sieff 4,7,8, Stuart H Orkin 4,7,8, David G Nathan 4,7,8, Eric S Lander 1,9,10, Hanna T Gazda 4,5
PMCID: PMC3386831  PMID: 22706301

Abstract

Diamond-Blackfan anemia (DBA) is a hypoplastic anemia characterized by impaired production of red blood cells, with approximately half of all cases attributed to ribosomal protein gene mutations. We performed exome sequencing on two siblings who had no known pathogenic mutations for DBA and identified a mutation in the gene encoding the hematopoietic transcription factor GATA1. This mutation, which occurred at a splice site of the GATA1 gene, impaired production of the full-length form of the protein. We further identified an additional patient carrying a distinct mutation at the same splice site of the GATA1 gene. These findings provide insight into the pathogenesis of DBA, showing that the reduction in erythropoiesis associated with the disease can arise from causes other than defects in ribosomal protein genes. These results also illustrate the multifactorial role of GATA1 in human hematopoiesis.

Introduction

Advances in genomic sequencing technology promise to provide a more complete picture of the genetic basis of human disease and to make new connections between molecular pathways involved in disease pathophysiology. Diamond-Blackfan anemia (DBA; OMIM 105650) is attributable to reduced proliferation and survival of erythroid progenitors leading to hypoproliferative anemia (1, 2). The anemia in DBA is characterized by the production of enlarged (macrocytic) erythrocytes and, unlike other anemias, by therapeutic response to corticosteroids. Over the past decade, the elucidation of mutations in the ribosomal protein gene RPS19 (3), followed by the discovery of mutations in 9 other ribosomal protein genes, has led to the hypothesis that DBA is a disorder of ribosomal biogenesis (1, 2). However, approximately 50% of DBA cases have as-yet-unidentified molecular mutations, despite systematic sequencing of all ribosomal protein and other candidate genes in these cases (1, 2, 4, 5). Recent work has highlighted the role of deletions of ribosomal protein genes that may be responsible for a subset of cases without previously identified mutations (6, 7). However, it is clear that the molecular etiology of many DBA cases remains to be uncovered. In light of this observation, we examined cases without previously identified pathogenic mutations in an attempt to identify new mutations that can cause DBA.

Results and Discussion

We focused on a family in which two male siblings were diagnosed with DBA (Figure 1A). While DBA generally demonstrates autosomal dominant inheritance (1), both parents in the family had entirely normal hematological analyses; assuming that the disease has full penetrance, this suggests X-linked or autosomal recessive inheritance. The affected siblings (II-1 and II-3) remain alive and most recently required chronic red blood cell transfusions for treatment (Table 1). Both siblings showed robust clinical responses to corticosteroid therapy for a period of 4 (II-1) and 6 (II-3) years, as is typical for DBA (Table 1). The siblings have macrocytic anemia, consistently low reticulocyte counts, and a modest elevation of fetal hemoglobin levels — features characteristic of DBA (Table 1 and Supplemental Table 1; supplemental material available online with this article; doi: 10.1172/JCI63597DS1). Sibling II-1 did not have an elevation of erythrocyte adenosine deaminase levels (Supplemental Table 1), which is seen in some DBA patients (1). Interestingly, sibling II-1 has also had a mildly low platelet count beginning at the age of 17 years, and both siblings were noted to have had occasional mild reductions in the neutrophil count, with those in sibling II-1 being consistently lower (Table 1). However, these siblings showed neither clinical signs of abnormal bleeding nor an increased propensity for infections. To confirm the clinical diagnosis of DBA, we reevaluated the original bone marrow aspirates and biopsies from these patients. Independent evaluation by hematopathologists agreed with the diagnosis of DBA. The bone marrow was noted to have erythroid hypoplasia without abnormalities of the other hematopoietic lineages (Figure 1, D–F).

Figure 1. Identification of GATA1 mutations in DBA.

Figure 1

(A) Pedigree of a family with DBA in 2 male children and normal hematological findings in the parents. (B) Sanger sequencing chromatograms from the 3′ end of exon 2 and 5′ end of intron 2 on GATA1 in the mother (I-2) and 3 children from the family shown in A. (C) RT-PCR analysis of GATA1 exons 1 and 3 from peripheral blood RNA samples from the patients (II-1 and II-3); their mother (I-2), who carries the GATA1 mutation; and a normal control. FL, full-length. (D and E) Bone marrow core sections from II-1 and II-3 shown at ×100 magnification demonstrate erythroid hypoplasia. (F) Rare erythroblasts with normal morphology were noted on bone marrow aspirates (from II-1; shown at ×100 magnification). (G) Sanger sequencing chromatograms show a GATA1 G nucleotide deletion (at the exon 2–intron 2 junction) in an independent male patient with DBA.

Table 1.

Hematologic parameters for index DBA cases

graphic file with name JCI63597.t1.jpg

We performed whole-exome sequencing on the 2 siblings with DBA, obtaining at least 10-fold coverage for more than 93% of the target bases (Supplemental Table 2 and refs. 8, 9). We reasoned that pathogenic mutations leading to DBA were likely to be rare in unaffected populations and therefore filtered out all variants identified from the latest draft of the 1000 Genomes Project, dbSNP build 132, and 95 exomes sequenced for the National Institute of Environmental Health Sciences Environmental Genome Project (Supplemental Table 2, Methods, and ref. 9). After filtering, a total of 74 variants were identified as being shared by the 2 affected siblings. We genotyped these mutations in the other family members (Figure 1A). Of the 74 mutations, 31 (42%) were found in the 2 affected siblings but not in an unaffected sibling (Supplemental Table 3). No variants were identified that would fit an autosomal recessive model of inheritance. Only a single variant on the X chromosome, within the GATA1 gene, showed appropriate segregation for an X-linked disorder with full penetrance (Figure 1, A and B, and Supplemental Table 3).

GATA1 encodes a transcription factor necessary for erythroid differentiation (10), and therefore it is biologically plausible that this gene is involved in DBA. The mutation in the GATA1 gene is a G→C transversion at position 48,649,736 on the X chromosome (hg19 coordinates) (Figure 1B) and results in the substitution of leucine for valine at amino acid 74 of the GATA1 protein. The mutation occurs at the last nucleotide of the exon 2 donor splice site and therefore would also be predicted to affect splicing of GATA1.

RT-PCR on peripheral blood–derived RNA samples from control individuals confirmed prior findings (11) that there are normally 2 splice variants of GATA1 produced: a full-length form involving splicing of exons 1, 2, and 3 with subsequent exons and a shorter GATA1s form involving splicing of exons 1 to 3 directly, with skipping of exon 2 (Figure 1C). By contrast, RT-PCR analysis of samples from the patients showed that the GATA1 mutation greatly favors the production of GATA1s mRNA, which lacks exon 2 (Figure 1C). Quantitative RT-PCR analysis of GATA1 exon 2 demonstrated that individuals II-1 and II-3 had only trace amounts of mRNA containing this exon (3%–5% of control levels), while their mother (I-2), who carries the GATA1 mutation, had a level at 53% of controls (Figure 2). This suggests that trace amounts of properly spliced full-length GATA1 mRNA may possibly be produced with this mutation. A lack of exon 2 would only allow translation to initiate at codon 84, resulting in the formation of the GATA1s protein that lacks the first 83 amino acids, which contain the transactivation domain of this transcription factor (Figure 3 and refs. 12, 13).

Figure 2. GATA1 exon 2 mutation results in trace amounts of GATA1 mRNA containing exon 2.

Figure 2

Quantitative RT-PCR was performed on peripheral blood RNA samples from individuals I-2, II-1, and II-3, as well as a normal control individual. Data are shown as the mean ± SD. Trace amounts of exon 2 are present in the male carriers of the GATA1 exon 2 mutation (3% and 5%, respectively), and a female carrier (I-2) with this mutation has half the level of mRNA compared with controls (53%).

Figure 3. A model of how GATA1 mutations in DBA favor production of GATA1s alone.

Figure 3

(A) Normal splicing pattern of GATA1 in humans and the resulting mRNA and protein products. (B) Aberrant splicing of exons 2 and 3 (highlighted by red star at mutation sites) leads to production of GATA1s alone. For the protein products, the transactivation domain (TD), N-terminal zinc finger (NF), and C-terminal zinc finger (CF) are shown.

We then sought to identify additional DBA patients carrying mutations in GATA1 by screening 62 additional male DBA patients without known pathogenic mutations. We identified one patient with a deletion of one of 2 adjacent G nucleotides (X chromosome positions 48,649,736–48,649,737) at the same genomic position as the GATA1 mutation found in the 2 brothers above (Figure 1G). This mutation would also be predicted to favor production of GATA1s, as a result of impaired splicing and frameshift of the full-length GATA1 open reading frame (Figure 1G). This patient has anemia that has responded to treatment with corticosteroids and has not had other hematologic abnormalities (Supplemental Table 4).

Interestingly, a mutation identical to the G→C transversion in exon 2 has been reported to result in dyserythropoietic anemia in humans, and other GATA1 germline mutations are associated with variable types of anemias and thrombocytopenias (11, 14, 15). These latter cases are due to missense mutations in the zinc fingers of GATA1 and are distinct from the mutations affecting the production of different isoforms (Figure 3). The variability among phenotypes seen in the different mutations favoring GATA1s production may be attributable to differences in the levels of GATA1 expressed. This phenomenon has been seen with mouse hypomorphic mutations, where even slight differences in Gata1 levels can lead to variable phenotypes involving survival defects, unrestrained proliferation, or impaired differentiation of erythroid progenitors (16, 17). We speculate that alterations in GATA1 expression may also underlie the phenotypic variability seen over time in the DBA patients. In addition, similar mutations that lead to the production of GATA1s alone are acquired somatically in all cases of Down syndrome–associated acute megakaryoblastic leukemia and transient myeloproliferative disease (12, 13). Mice with a mutation resulting in expression of only GATA1s have apparently normal erythropoiesis (18), which emphasizes the species-divergent functions of GATA1. Specifically, these findings demonstrate that the full-length form of GATA1 is required for normal erythropoiesis in humans, but not in mice.

Systematic sequencing of GATA1 mutations in other cases of DBA will likely unveil similar mutations and reveal the extent to which such mutations contribute to this disease. All 3 of the patients with GATA1 mutations meet all of the current clinical diagnostic criteria for DBA and many of the supportive criteria, with the exception of elevations in erythrocyte adenosine deaminase levels (19). However, discovery and further phenotypic analysis of DBA patients with GATA1 mutations may uncover unique differences between this set of patients and cases due to ribosome protein gene mutations, which may lead to revision of the current diagnostic criteria for DBA (19). While the majority of studies on DBA pathogenesis have been focused on the role of ribosomal biogenesis, the finding of GATA1 mutations in DBA opens new avenues for studying the underlying basis of this disorder. These findings may provide insight into the erythroid specificity of this disease, which remains an enigma. Additionally, these DBA cases, coupled with the phenotypes described for other human GATA1 mutations (11, 14, 15), increase our understanding of how this transcription factor plays a role in specifying human erythropoiesis.

Methods

Exome sequencing and analysis.

The DBA patient cohort has been described previously (4, 5). All patients were selected based on the diagnosis of DBA, using criteria outlined previously (1). Exome sequencing was performed at the Broad Institute (8, 9). Briefly, oligonucleotides with 170 bp of target sequence flanked by 15 bp of universal primer sequence were synthesized in parallel on an Agilent microarray and subsequently cleaved. The oligonucleotides were PCR amplified and transcribed in vitro with biotinylated UTP to generate single-stranded RNA “bait.” The genomic DNA was sheared, ligated to sequencing adapters, and selected for lengths between 200 and 350 bp. This “pond” of DNA was hybridized with an excess of bait in solution. The captured material was pulled down by magnetic beads coated with streptavidin and subsequently eluted. Afterward, each sample was pooled, and sufficient sequencing was performed so that each sample had an average coverage equivalent to one lane of sequencing with 76-bp paired-end reads using an Illumina HiSeq 2000 sequencer.

All sequencing data were processed through an automated analysis pipeline built around the Picard suite ( http://picard.sourceforge.net/), and BAM files were exported from this process (using the hg19 human genome draft). These BAM files were then run through a variant caller pipeline utilizing the Genome Analysis Toolkit (GATK) (20). This pipeline implements best-practice approaches for SNP and indel calling, and variants for each individual sample were compiled into a single variant call format (VCF) file.

Once all variants were obtained, annotated, and assessed from the exome sequencing process, variant filtration was performed. We gathered data for all variants from the June 2011 data release of the 1000 Genomes Project (21) ( http://www.1000genomes.org/), dbSNP build 132 ( http://www.ncbi.nlm.nih.gov/projects/SNP/), and 95 exomes available from the National Institute of Environmental Health Sciences Environmental Genome Project ( http://evs.gs.washington.edu/niehsExome/). We filtered variants in the patient samples using all of these datasets with the GATK Variant Filtration and Select Variants packages (20). Metrics from this process are shown in Supplemental Table 2. We developed custom Perl scripts to assess the number of variants in various functional classes following variant filtration. We also developed a custom Perl script to assess common variants that were identified in both siblings affected with DBA.

Sanger sequencing–based genotyping of variants.

A custom Perl script was written to design primer pairs for all variants identified from the analysis described above to genotype all affected and unaffected family members (5 total individuals). We used the script to get the genomic sequence surrounding the variant and then used the Primer3 program ( http://frodo.wi.mit.edu/primer3/) to design primers to amplify a fragment of 200–300 bp centered around each variant. The same set of primers was used for both PCR amplification from genomic DNA samples and for Sanger sequencing. Results from the sequencing-based genotyping were curated using automated and manual approaches. The results of the genotyping for all 5 family members are listed in Supplemental Table 3. Sixty-two additional male patients with DBA were screened for GATA1 mutations. All 6 exons of GATA1 were screened for mutations using standard PCR-based Sanger sequencing.

RT-PCR analysis.

Total RNA was isolated from peripheral blood using a Paxgene Blood RNA kit (QIAGEN/BD) and treated with DNase (QIAGEN). RT-PCR was performed using a One-Step RT-PCR kit (QIAGEN). RT-PCR primers were designed in exon 1 (forward, 5′-ACACTGAGCTTGCCACATC-3′) and in exon 3 (reverse, 5′-CACAGTTGAGGCAGGGTAGAG-3′) of GATA1. RT-PCR was performed for 30 cycles with an annealing temperature of 57°C, and the products were analyzed by agarose gel electrophoresis.

Quantitative RT-PCR.

To detect expression of GATA1 exon 2, RNA was isolated from peripheral blood as above. cDNA was prepared using the SuperScript III First-Strand Synthesis System for RT-PCR (Invitrogen). Real-time PCR for GATA1 exon 2 was performed using the SYBR Green PCR Master Mix (Applied Biosystems) and Applied Biosystems Real-Time PCR 7300 System. GAPDH was used as the control to normalize GATA1 exon 2 expression levels. GATA1 expression quantification was performed using the ΔΔCt method (22). The following primers were used for quantitative RT-PCR: GATA1 exon 2, forward 5′-CCCCAGTTTGTGGATCCTG-3′, reverse 5′-ACCCCTGATTCTGGTGTGG-3′; GAPDH, 5′-TGCACCACCAACTGCTTAGC-3′, reverse 5′-GGCATGGACTGTGGTCATGAG-3′.

Statistics.

All pairwise comparisons were assessed using unpaired 2-tailed Student t test. Results were considered significant if the P value was less than 0.05.

Study approval.

All patients or their families had provided written informed consent to participate in this study. The institutional review boards at the Massachusetts Institute of Technology/Broad Institute and the Children’s Hospital Boston approved the study protocols.

Supplementary Material

Supplemental data
JCI63597sd.pdf (1.4MB, pdf)

Acknowledgments

We are grateful to the families involved in this work for their courage and commitment to research and to the clinicians caring for these patients. We thank M. Ilzarbe, N. Gupta, J. Murphy, and S. Flynn for their assistance in study organization; M. DePristo, C. Hartl, and K. Shakir for assistance with genetic analysis; H. Lodish, L. Ludwig, O. Zuk, M. Garber, and M. Schnall-Levin for valuable comments and assistance; and T. DiCesare for assistance with illustrations. This work was supported by NIH grant T32 HL007574-30 (to V.G. Sankaran); NIH grant R01 HL107558 and grants from the Manton Center for Orphan Disease Research and the Diamond-Blackfan Anemia Foundation (to H.T. Gazda); and NIH grant U54 HG003067-09 (to E.S. Lander).

Footnotes

Conflict of interest: The authors have declared that no conflict of interest exists.

Citation for this article: J Clin Invest. 2012;122(7):2439–2443. doi:10.1172/JCI63597.

See the related Commentary beginning on page 2346.

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Associated Data

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Supplementary Materials

Supplemental data
JCI63597sd.pdf (1.4MB, pdf)

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