Acquisition of loss of the wild-type NRAS locus with aggressive disease progression in a patient with juvenile myelomonocytic leukemia and a heterozygous NRAS mutation

doi:10.3324/haematol.11503

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Juvenile Myelomonocytic Leukemia

Acquisition of loss of the wild-type NRAS locus with aggressive disease progression in a patient with juvenile myelomonocytic leukemia and a heterozygous NRAS mutation

Kazuyuki Matsuda^*, Yozo Nakazawa^°, Kazuo Sakashita^°, Masaaki Shiohara^°, Kazuyoshi Yamauchi^*, Kenichi Koike^°^,

^* Department of Laboratory Medicine, Shinshu University Hospital, Matsumoto;
^° Department of Pediatrics, Shinshu University School of Medicine, Matsumoto, Japan

Correspondence: Kenichi Koike, M.D., Department of Pediatrics, Shinshu University School of Medicine, 3-1-1, Asahi, Matsumoto, 390-8621, Japan. Phone: international +81.263372642. Fax: international +81.263373089. E-mail: koikeken{at}hsp.md.shinshu-u.ac.jp

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In a patient with juvenile myelomonocytic leukemia, a NRAS mutationat codon 12 (GGT>TGT) was initially heterozygous, but becamehomozygous after blastic crisis (BC). According to microsatelliteand FISH analyses, the post-BC homozygous mutation might resultfrom the loss of the wild-type NRAS locus through mitotic recombination.

Key words: JMML, NRAS mutation, blastic crisis, LOH, mitotic recombination.

Somatic point mutations of the RAS genes are found in approximately25% of patients with juvenile myelomonocytic leukemia (JMML).¹Although at present allogeneic hematopoietic stem cell transplantationis the only curative treatment for JMML, high relapse rate isa serious problem. Among variables analyzed, transformationto acute leukemia, often referred to as blastic crisis (BC),at the time of transplantation was associated with increasedcumulative incidence of post-transplant relapse.² The geneticmechanism underlying BC, however, remains to be determined.

A 2-month old boy was diagnosed as having JMML and treated with6-mercaptopurine. After 2 years, the laboratory findings revealeda marked leukocytosis, thrombocytopenia, and 43% blasts in bonemarrow. The blasts were positive for myeloperoxidase, alpha-naphthylbutylate esterase, and CD13/CD33, indicating progression towardmyeloid BC. Three months later, chromosomal analysis of thebone marrow cells showed the advent of monosomy 7. The detailsof the clinical course have been previously reported.³

A single nucleotide substitution at codon 12 of the NRAS genefrom GGT to TGT was detected with the concomitant normal sequencein peripheral blood mononuclear cells (PB MNCs) obtained beforetreatment with 6-mercaptopurine, as shown in Figure 1A. Therewere no mutations at codons 12, 13, and 61 of the KRAS2 geneor at exons 3, 8, and 13 of the PTPN11 gene. However, PB MNCsobtained 5 months after BC showed the homozygous NRAS mutation(GGT>TGT). Mutant allele-specific amplification (MASA) analysiswas then performed on PB-derived granulocyte-macrophage (GM)colony-constituent cells generated with GM colony-stimulatingfactor (CSF) and stem cell factor (SCF) in a methylcelluloseculture.⁴ As shown in Figure 1B, both the mutant PCR productand the wild-type product were detected in all of 11 GM colony-constituentcells before BC. By contrast, only the mutant product was amplifiedfrom all of 24 GM colony-constituent cells after BC. Thus, thepatient’s malignant myeloid lineage cells might initiallypossess the heterozygous NRAS mutation and might subsequentlyacquire the homozygous NRAS mutation. Using microsatellite analyses,we attempted to verify whether the homozygous NRAS mutationafter BC was due to loss of heterozygosity (LOH) related tothe NRAS gene according to the procedure previously described.⁵Since there were no polymorphic microsatellite markers insidethe NRAS gene, we used three microsatellite markers (D1S250,D1S2687 and D1S189) near the gene on the short arm of chromosome1p13 (Figure 2A). D1S468, 112 Mb downstream from the NRAS gene,was used as a control. We made 9 pairs of pre-BC and post-BCGM colony samples whose sequences were all determined by theMASA method, and then compared numbers of the dinucleotide repeatsin the marker DNAs. As shown in Figure 2B, the ratio of P1:P2in post-BC/P1:P2 in pre-BC of D1S250 was higher than 1.35 (27.25±1.57,mean±SD). Ratios of post-P1:P2/pre-P1:P2 in D1S2687 andD1S189 were less than 0.67 (0.26±0.05 and 0.37±0.04,respectively). By contrast, the ratio of post-P1:P2/pre-P1:P2in D1S468 was 0.85±0.05. Thus, these results suggestthat LOH related to the NRAS locus joined the heterozygous NRASmutation after BC. Finally, we examined the mechanism of theLOH. FISH analysis (using probes for the region containing theNRAS gene on chromosome 1p13 and for the region containing D1S468on chromosome 1p36)^6,7 and MASA assay were simultaneously performedon post-BC GM colony-constituent cells generated with GM-CSFand SCF. Thirteen out of 30 GM colonies with the homozygousmutation contained 1–2 metaphase cells per colony. Ineach of the 23 metaphase cells examined, the signals for RP5-1000E10encompassing the NRAS gene were found on both chromosome 1 homologs(Figure 2C). These results suggest that the LOH resulted fromduplication of the mutated allele through mitotic recombination,rather than from deletion of the NRAS part of wild-type chromosome1p.

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Figure 1. Mutation analyses of the NRAS gene (A). The direct sequencing traces showing codon 12 of the NRAS gene in PB cells before and after blastic crisis (BC) of the patient. The heterozygous mis-sense mutation was observed before BC, whereas the homozygous mutation was observed after BC. (B) Data show PCR products of the mutated and/or wild-type NRAS alleles obtained from PB-MNCs of 4 normal controls, 6 pre-BC GM colony-constituent cells and 6 post-BC GM colony-constituent cells of the present case with codon 12 GGT $->$ TGT mutation, and 6 GM colony-constituent cells of another case with codon 12 GGT $->$ AGT mutation, using the MASA method. This latter case was used to show the reliability of our mutant allele-specific amplification technique. Primers 5'-CTGGTGGTG-GTTGGAGCAT-3' and NRAS-R (5'-TCCGACAAGTGAGAGACAGG-3'), were used to detect the mutant NRAS sequence (GGT $->$ TGT), whereas the primers 5'-TGGTGGTG-GTTGGAGCAG-3' and NRAS-R, were used to detect the wild-type NRAS sequence. For the other mutant NRAS sequence (GGT $->$ AGT), we used the primers 5'-CTGGTGGTG-GTTGGAGCAA-3' and NRAS-R. GGT, wild-type allele; TGT, GGT $->$ TGT mutant allele; AGT, GGT $->$ AGT mutant allele.

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Figure 2. LOH analyses of the NRAS gene. (A) Chromosome 1p showing the markers used for microsatellite PCR analysis and FISH. (B) Analyses of polymorphic microsatellite marker DNAs on the short arm of chromosome 1 We made 9 pairs of pre-blastic crisis (BC) and post-BC GM colony samples (sequences were all determined by the MASA method), and then compared numbers of the dinucleotide repeats in 4 marker DNAs: D1S250, 40kb downstream from the NRAS gene; D1S2687 and D1S189, 1 Mb and 1.5 Mb upstream to the gene, respectively; D1S468, 112 Mb downstream from the NRAS gene. The forward primers were labeled with a fluorescence dye marker (5-6-carboxyfluorescein). Alleles were defined as the two highest peaks (P1 and P2) within the expected size range. Numbers within the rectangle indicate the size of the short tandem repeat (STR), and numbers below the rectangles indicate the height of the STR peaks. According to the maufacurer’s instructions, when the ratio of P1:P2 in the post-BC sample/P1:P2 in the pre-BC sample was either less than 0.67 or greater than 1.35, a LOH was confirmed.

C. FISH analysis using probes for the region containing the NRAS gene on chromosome 1p13 and for the region containing D1S468 on chromosome 1p36 was performed on post-BC GM colony-constituent cells generated with GM-CSF and SCF. Orange signals, RP5-1000E10 encompassing the NRAS gene; green signals, RP5-1092A11 encompassing D1S468. On a metaphase cell, the orange signals were recognized on both chromosome 1 homologs.

Braun et al.⁸ reported that somatic activation of a latent KRAS^G12Dallele rapidly induces a fatal myeloproliferative disorder inmice. However, our recent study revealed hematologic improvementdespite no chemotherapy during a 2- to 4-year follow-up in JMMLpatients with a NRAS or KRAS2 glycine to serine substitution,⁹implying that all types of RAS mutations are not always sufficientto confer the disease progression. Given the results of a 7,12-dimethylbenz[a]anthracene-inducedrat leukemia model,¹⁰ the two stages of genetic change in ourcase suggest that oncogenic heterozygous RAS mutations are anearly event of leukemogenesis, but in JMML the aggressive developmentrequires other genetic lesions.

Footnotes

Funding: this work was supported by Grants-in-Aid No. 11390300from the Ministry of Education of Japan.

References

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ABSTRACT
References

Lauchle JO, Braun BS, Loh ML, Shannon K. Inherited predispositions and hyperactive Ras in myeloid leukemogenesis. Pediatr Blood Cancer 2006;46:579-85.[CrossRef][ISI][Medline]
Locatelli F, Nöllke P, Zecca M, Korthof E, Lanino E, Peters C, et al. Hematopoietic stem cell transplantation (HSCT) in children with juvenile myelomonocytic leukemia (JMML): results of the EWOG-MDS/EBMT trial. Blood 2005;105:410-9.
Nakazawa T, Koike K, Agematsu K, Itoh S, Hagimoto R, Kitazawa Y, et al. Cytogenetic clonality analysis in monosomy 7 associated with juvenile myelomonocytic leukemia: clonality in B and NK cells, but not in T cells. Leuk Res 1998;22:887-92.[CrossRef][ISI][Medline]
Sakashita K, Koike K, Kinoshita T, Shiohara M, Kamijo T, Taniguchi S, et al. Dynamic DNA methylation change in the CpG island region of p15 during human myeloid development. J Clin Invest 2001;108:1195-204.[CrossRef][ISI][Medline]
Matsuda K, Yamauchi K, Tozuka M, Suzuki T, Sugano M, Hidaka E, et al. Monitoring of hematopoietic chimerism using short tandem repeat, and effect of CD selection upon its sensitivity. Clin Chem 2003;50:2411-4.[CrossRef][ISI]
Kobayashi N, Matsuda K, Sakashita K, Matsuzaki S, Iwasaki R, Koike K. Bilineage acute leukemia of T-lymphoid and myeloid lineages. Haematologica 2004;89:1139-41.[Abstract/Free Full Text]
Baxter EJ, Scott LM, Campbell PJ, East C, Fourouclas N, Swanton S, et al. Acquired mutation of the tyrosine kinase JAK2 in human myeloproliferative disorders. Lancet 2005;365:1054-61.[ISI][Medline]
Braun BS, Tuveson DA, Kong N, Le DT, Kogan SC, Rozmus J, et al. Somatic activation of oncogenic Kras in hematopoietic cells initiates a rapidly fatal myeloproliferative disorder. Proc Natl Acad Sci USA 2004;101:597-602.[Abstract/Free Full Text]
Matsuda K, Shimada A, Yoshida N, Ogawa A, Watanabe A, Yajima S, et al. Spontaneous improvement of hematologic abnormalities in patients having juvenile myelomonocytic leukemia with specific RAS mutations. Blood 2007;109:5477-80.[Abstract/Free Full Text]
Osaka M, Matsuo S, Koh T, Sugiyama T. Loss of heterozygosity at the N-ras locus in 7,12-dimethylbenz[a] anthracene-induced rat leukemia. Mol Carcinog 1997;18:206-12.[CrossRef][ISI][Medline]

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