Abstract
DEAD-box proteins comprise a family of ATP-dependent RNA helicases involved in several aspects of RNA metabolism. Here we report the characterization of the human DEAD-box RNA helicase DDX26. The gene is composed of 14 exons distributed over an extension of 8,123 bp of genomic sequence and encodes a transcript of 1.8 kb that is expressed in all tissues evaluated. The predicted amino acid sequence shows a high similarity to a yeast DEAD-box RNA helicase (Dbp9b) involved in ribosome biogenesis. The new helicase maps to 7p12, a region of frequent chromosome amplifications in glioblastomas involving the epidermal growth factor receptor (EGFR) gene. Nevertheless, co-amplification of DDX26 with EGFR was not detected in nine tumors analyzed.
DDX26; DEAD-box RNA helicase; 7p12; ribosome biogenesis
Braz J Med Biol Res, October 2001, Volume 34(10) 1237-1245
Molecular characterization of DDX26, a human DEAD-box RNA helicase, located on chromosome 7p12
A.A. Camargo1, D.N. Nunes1, H.B. Samaia1, L. Liu2, V.P. Collins2, A.J.G. Simpson1 and E. Dias-Neto1
1Instituto Ludwig de Pesquisa sobre o Câncer, São Paulo, SP, Brasil
2Department of Histopathology, University of Cambridge, Addenbrooke's Hospital, Cambridge, UK
References
Correspondence and Footnotes Correspondence and Footnotes Correspondence and Footnotes
Abstract
DEAD-box proteins comprise a family of ATP-dependent RNA helicases involved in several aspects of RNA metabolism. Here we report the characterization of the human DEAD-box RNA helicase DDX26. The gene is composed of 14 exons distributed over an extension of 8,123 bp of genomic sequence and encodes a transcript of 1.8 kb that is expressed in all tissues evaluated. The predicted amino acid sequence shows a high similarity to a yeast DEAD-box RNA helicase (Dbp9b) involved in ribosome biogenesis. The new helicase maps to 7p12, a region of frequent chromosome amplifications in glioblastomas involving the epidermal growth factor receptor (EGFR) gene. Nevertheless, co-amplification of DDX26 with EGFR was not detected in nine tumors analyzed.
Key words: DDX26, DEAD-box RNA helicase, 7p12, ribosome biogenesis
Introduction
Helicases, including DNA and RNA helicases, are grouped into two major superfamilies of proteins (SFI and SFII) on the basis of the occurrence of conserved motifs (1). RNA helicases are mostly of the SFII superfamily and can be further classified into families on the basis of particular consensus sequences in the conserved ATP hydrolysis motif. In contrast to DNA helicases, which processively unwind long regular dsDNA structures, most RNA helicases modulate only short duplex regions in RNA molecules in a one-step reaction in the presence of ATP (1).
RNA helicases are involved in various steps of RNA metabolism including transcription, pre-mRNA splicing, ribosome biogenesis, cytoplasmic transport, translation, initiation/elongation, and mRNA decay (1). DEAD-box RNA helicases are characterized by the presence of eight conserved motifs including an RNA interaction domain and an ATP hydrolysis motif containing the core amino acid sequence DEAD (2). In addition to the conserved motifs, RNA helicases contain variable N and C terminal extensions that might confer substrate specificity and/or contain information directing subcellular localization (3).
Chromosome amplifications and overexpression of different DEAD-box RNA helicases have already been reported in different tumors (4-7), suggesting a general role for RNA helicases in tumorigenesis. Here we report the chromosomal localization, genomic organization and expression of DDX26, a human DEAD-box RNA helicase, with high similarity to an essential yeast RNA helicase (Dbp9b) involved in the assembly of early pre-ribosomal particles. The new helicase maps to 7p12, a region of frequent chromosome amplifications in glioblastomas involving the epidermal growth factor receptor (EGFR) gene. Nevertheless, co-amplification of DDX26 with EGFR was not detected in nine tumors analyzed.
Material and Methods
Computational prediction of gene structure
Gene structure was predicted by tBlastN analysis using the yeast orthologous protein Dbp9b as a query. Proximal and distal exons were then predicted by BlastN analysis using the PAC sequence (AC004938) as a query against human ESTs available in dbEST (AW250279, AI242741). Oligonucleotides corresponding to the 5' and 3' ends of the putative transcript (Figure 1A) were designed and used to amplify cDNAs derived from colon and breast tumors by PCR. Intron/exon boundaries were determined by aligning the cDNA sequence with the genomic sequence from the PAC clone.
[View larger version of this image (433 K JPG file)]
RT-PCR and sequencing
Total RNA was extracted from breast and colon tumors using Trizol reagent (Gibco-BRL, Gaithersburg, MD, USA) following manufacturer's instructions. Two micrograms of total RNA was reverse-transcribed into first-strand cDNA using SuperScript II and oligo dT in a final volume of 20 µl. PCR was carried out in a 10-µl reaction mixture containing 1 µl of cDNA, 1X Taq DNA polymerase buffer, 200 µM dNTPs, 2 pmol of each primer and 1 U Taq DNA polymerase (Gibco-BRL). Cycling conditions were 94oC for 5 min, followed by 40 cycles of 94oC for 1 min, 60oC for 1 min, 72oC for 2 min and a final extension at 72oC for 10 min. PCR products were analyzed on ethidium bromide-stained agarose gels before sequencing. PCR products were used directly in sequencing reactions with Big Dye terminator mix on an ABI377 sequencer according to manufacturer's instructions. Sequencing reactions were performed with the same primers used for RT-PCR and internal primers as indicated in Figure 1.
Northern and dot blot hybridization
A commercial "Human Master Blot" (Clontech, Palo Alto, CA, USA) containing normalized loading of polyA+ RNA from 75 different human tissues and a "Cancer Cell Lines Northern blot" (Clontech) containing 2 µg of polyA+ RNA was used for evaluating DDX26 expression. A 32P-labeled probe corresponding to the 3' end of the transcript was hybridized in 5 ml ExpressHyb solution (Clontech) at 65oC overnight. The membranes were washed twice with 2X SSC/0.1% SDS at room temperature for 5 min and then twice with 2X SSC/0.1% SDS for 20 min at 65oC before exposure at -70oC for 24 h.
Southern blotting and densitometry
Allele dosage at the DDX26 locus was quantitated by Southern blotting in a panel of nine glioblastomas with known 7p12 amplifications. Southern blotting, hybridization and PhosporImage analysis were performed as previously described (8). Probes used for hybridizations were: WI-15640, SGC34528, D7S2542, WI-6548, EGFR, SGC32574, WI-18503, WI-16990, SHGC11828 and a 1.2-kb fragment from the 3' end of DDX26 transcript.
Results
As part of the Ludwig/FAPESP Human Cancer Genome Project (9), we identified an EST with significant similarity to a DEAD-box RNA helicase from yeast and various other organisms as well as to a finished human genomic sequence corresponding to the PAC clone DJ0971C03 (AC004938). Matches with previously known human helicases, however, were found to be only marginal, indicating that this EST is a new member of the DEAD-box family not annotated in the PAC sequence.
We have used the yeast orthologous gene to search for the human genomic sequence and to predict gene structure. Primers for RT-PCR amplification were designed for validation and sequencing of the predicted transcript. As expected from the computational prediction, a 1,889-bp fragment was obtained by RT-PCR and fully sequenced by primer walking (Figure 1A). This gene was named DDX26 after consulting the HUGO Genome Nomenclature Committee and deposited in GenBank (AF247666). The gene consists of 14 exons distributed over an extension of 8,123 bp of genomic sequence. Exons and introns vary in size from 74 to 275 bp and from 92 to 1,594 bp, respectively (Figure 1B). Computer analysis of the PAC sequence using Genscan failed to predict the correct gene structure due to the apparent existence of other genes in the same region and to the small size of exon 13 that was not detected by using this program.
Complete sequencing of this helicase revealed a single putative open reading frame coding for a protein of 548 amino acids (Figure 1A). Analysis of the predicted protein sequence using Pfam (http://pfam. wustl.edu/) revealed the presence of two highly conserved domains corresponding to a DEAD/DEAH-box helicase domain (20-234 amino acids) and a helicase C-terminal conserved domain (272-380 amino acids). Figure 2 shows the alignment of the predicted amino acid sequence of DDX26 with RNA helicases from Drosophila, yeast, Candida and the human DDX6 using CLUSTAL W (10). As for the first EST, a high similarity was observed with an essential yeast RNA helicase (Dbp9b) involved in the assembly of early pre-ribosomal particles (43% identity and 64% similarity). The putative function of this protein in ribosome biogenesis was recently confirmed by Zirwes and colleagues (11) during the preparation of this manuscript.
To determine the pattern of expression of DDX26 in different human tissues, a 1.5-kb cDNA fragment corresponding to the 3' portion of the mRNA was hybridized against commercial filters (Clontech) (Figure 3). While dot blot analysis indicated a ubiquitous expression of DDX26 in all tissues analyzed, a more detailed analysis showed a higher expression in cerebellum, pituitary gland, fetal kidney and fetal lung (Figure 3A). The specificity of the dot blot signal was confirmed by Northern blot analysis which showed the presence of a band of the expected size in all tumor cell lines tested. The highest expression level was observed in the melanoma cell line G-361 (Figure 3C). No alternative splicing forms were evident by Northern blot or Blast analysis against human ESTs.
The PAC clone was mapped to human chromosome 7p12, a region of frequent chromosome rearrangements in glioblastomas (12). The EGFR gene is located in this same region which is amplified in 40% of glioblastomas together with extensive amplicons including a number of adjacent loci in some of these tumors. Five percent of 7p12 amplicons do not include EGFR, suggesting that other still unidentified genes at this locus may be amplified in glioblastomas (8). Southern blotting and densitometry were used to test the possible amplification of this human RNA helicase in tumors. As shown in Table 1, of nine glioblastoma analyzed, eight have amplifications of the EGFR locus, but co-amplification of DDX26 was not detected in any of them.
[View larger version of this image (271 K JPG file)]
[View larger version of this image (97 K GIF file)]
Discussion
DDX26, a human RNA helicase from the DEAD-box family, was cloned and characterized based on similarity to a yeast orthologous gene Dbp9b. Cross-species sequence comparison was shown to be a useful tool for identification of exons due to their strong conservation during evolution when compared with random genomic sequences. Accordingly, we have used the yeast orthologous gene to search the human genomic sequence and to predict gene structure. Primers for RT-PCR amplification were designed for validation and sequencing of the predicted transcript.
Complete sequencing of the 1,889-bp PCR fragment revealed a single putative open reading frame coding for a protein of 548 amino acids with high similarity to an essential yeast RNA helicase (Dbp9b) involved in the assembly of early pre-ribosomal particles. The corresponding transcript is expressed in a broad range of tissues in agreement with the putative functional role in ribosome biogenesis.
DDX26 is located on chromosome 7p12, a region of frequent chromosome rearrangements in glioblastomas (12). The EGFR gene is located in this same region which is amplified in 40% of glioblastomas together with extensive amplicons including a number of adjacent loci in some of these tumors. Recently, Wang et al. (13) described a new gene coding for a putative tyrosine kinase substrate (GBAS) that was co-amplified with EGFR in 2 of 12 tumors and in 2 of 3 cell lines analyzed.
Chromosome rearrangements, amplifications and overexpression of different DEAD-box RNA helicases have already been reported for different tumors (4-7). Nevertheless, co-amplification of DDX26 was not detected in eight tumors with amplification at the EGFR locus, excluding the involvement of this helicase in glioblastoma development.
Acknowledgments
We thank Dr. Ricardo R. Brentani for continuous support and for a critical reading of the manuscript. We also thank Elaine Pereira Guimarães for technical assistance.
Address for correspondence: A.A. Camargo, Instituto Ludwig de Pesquisa sobre o Câncer, Rua Prof. Antônio Prudente, 109, 4º andar, 01509-010 São Paulo, SP, Brasil. Fax: +55-11-270-7001. E-mail: anamaria@compbio.ludwig.org.br
D.N. Nunes and H.B. Samaia are recipients of FAPESP fellowships. The sequence described was deposited in GenBank under accession No. AF247666. Received February 1, 2001. Accepted June 28, 2001.
- 1. de La Cruz J, Kressler D & Linder P (1999). Unwinding RNA in Saccharomyces cerevisiae: DEAD-box proteins and related families. Trends in Biochemical Sciences, 24: 192-198.
- 2. Schmid SR & Linder P (1992). D-E-A-D protein family of putative RNA helicases. Molecular Microbiology, 6: 283-391.
- 3. Wang Y & Guthrie C (1998). PRP16, a DEAH-box RNA helicase, is recruited to the spliceosome primarily via its nonconserved N-terminal domain. RNA, 4: 1216-1229.
- 4. Akao Y, Seto M, Yamamoto K, Iida S, Nakazawa S, Inazawa J, Abe T, Takahashi T & Ueda R (1992). The RCK gene associated with t(11;14) translocation is distinct from the MLL/ALL-1 gene with t(4;11) and t(11;19) translocations. Cancer Research, 52: 6083-6087.
- 5. Amler LC, Schurmann J & Schwab M (1996). The DDX1 gene maps within 400 kbp 5' to MYCN and is frequently coamplified in human neuroblastoma. Genes, Chromosomes and Cancer, 15: 134-137.
- 6. Arai Y, Hosoda F, Kobayashi H, Arai K, Hayashi Y, Kamada N, Kaneko Y & Ohki M (1997). The inv(11)(p15q22) chromosome translocation of de novo and therapy-related myeloid malignancies results in fusion of the nucleoporin gene, NUP98, with the putative RNA helicase gene, DDX10. Blood, 89: 3936-3944.
- 7. Ishiguro T, Nakajima M, Naito M, Muto T & Tsuruo T (1996). Identification of genes differentially expressed in B16 murine melanoma sublines with different metastatic potentials. Cancer Research, 56: 875-879.
- 8. Liu L, Ichimura K, Pettersson EH & Collins VP (1998). Chromosome 7 rearrangements in glioblastomas; loci adjacent to EGFR are independently amplified. Journal of Neuropathology and Experimental Neurology, 57: 1138-1145.
- 9. Dias-Neto E, Garcia CR, Verjovski-Almeida S, Briones MR, Nagai MA, da Silva WJ, Zago MA, Bordin S, Costa FF, Goldman GH, Carvalho AF, Matsukuma A, Baia GS, Simpson DH, Brunstein A, de Oliveira PS, Bucher P, Jongeneel CV, O'Hare MJ, Soares F, Brentani RR, Reis LF, de Souza SJ & Simpson AJ (2000). Shotgun sequencing of the human transcriptome with ORF expressed sequence tags. Proceedings of the National Academy of Sciences, USA, 97: 3491-3496.
- 10. Thompson JD, Higgins DG & Gibson TJ (1994). CLUSTAL W: improving the sensitivity of progressive multiple sequence alignment through sequence weighting, position-specific gap penalties and weight matrix choice. Nucleic Acids Research, 22: 4673-4680.
- 11. Zirwes RF, Eilbracht J, Kneissel S & Schmidt-Zachmann MS (2000). A novel helicase-type protein in the nucleolus: protein NOH61. Molecular Biology of the Cell, 11: 1153-1167.
- 12. Chaffanet M, Chauvin C, Laine M, Berger F, Chedin M, Rost N, Nissou MF & Benabid AL (1992). EGF receptor amplification and expression in human brain tumours. European Journal of Cancer, 28: 11-17.
- 13. Wang XY, Smith DI, Liu W & James CD (1998). GBAS, a novel gene encoding a protein with tyrosine phosphorylation sites and a transmembrane domain, is co-amplified with EGFR. Genomics, 49: 448-451.
Correspondence and Footnotes
Publication Dates
-
Publication in this collection
02 Oct 2001 -
Date of issue
Oct 2001
History
-
Accepted
28 June 2001 -
Received
01 Feb 2001