Abstract
Despite having several characteristics of naı̈ve B cells, chronic lymphocytic leukemia (CLL) cells have been shown in some cases to have somatically mutated Ig variable region genes, indicating that the cell of origin has passed through the germinal center. A previous study of patients with CLL found an association between lack of somatic mutation and trisomy 12 and, therefore, possibly with a less favorable prognosis. We have sequenced the Ig VH genes of the tumor cells of 84 patients with CLL and correlated our findings with clinical features. A total of 38 cases (45.2%) showed ≥ 98% sequence homology with the nearest germline VH gene; 46 cases (54.8%) showed >2% somatic mutation. Unmutated VH genes were significantly associated with V1-69 and D3-3 usage, with atypical morphology; isolated trisomy 12, advanced stage and progressive disease. Survival was significantly worse for patients with unmutated VH genes irrespective of stage. Median survival for stage A patients with unmutated VH genes was 95 months compared with 293 months for patients whose tumors had mutated VHgenes (P = .0008). The simplest explanation is that CLL comprises 2 different diseases with different clinical courses. One, arising from a memory B cell, has a benign course, the other, arising from a naı̈ve B cell, is more malignant.
CHRONIC LYMPHOCYTIC leukemia (CLL) is characterized by the relentless accumulation of monoclonal B cells with the appearance of small mature lymphocytes and with a characteristic immunophenotype. Typically, they are positive for CD5, CD23, and CD19 and negative for surface CD22 and FMC7.1 Surface Ig (usually IgM plus IgD) is sparse and the immunoglobulin-associated molecule, CD79b, is low or absent.2 Most cells are in the G0 phase of the cell cycle and are unresponsive to mitogenic stimuli.3The cells overexpress the Bcl-2 gene product and are resistant to apoptosis.4
Because CD5 positive B cells are found in the fetal spleen5and surface IgD is a feature of cells that have not yet met antigen in the germinal center,6 it has been suggested that CLL is a tumor of naı̈ve B cells possibly arising in the follicular mantle zone.7
A further means of establishing the stage of differentiation of a B lymphocyte is provided by examining the Ig variable domain genes. Although the selection and recombination of VH, D, and JH genes and the insertion of nontemplated nucleotides at the VH-D and D-JH junctions are early events occurring in the bone marrow, the process of somatic mutation, which tends to focus amino acid changes in the first and second complementarity determining regions (CDR1 and CDR2) of the molecule, occurs in the germinal center environment.8
Early sequences of the VH genes of tumor cells from patients with CLL found them to be in germline configuration,9-11 tending to confirm their origin from a naı̈ve B cell. However, reports began to appear in the literature detailing cases with evidence of somatic mutation culminating in 1994 with a review of the literature by Schroeder and Dighiero,12 which found that 36 of 75 reported cases had VH genes with less than 98% sequence homology to the appropriate germline gene. The figure of 98% was chosen because polymorphisms, which are quite common in VH genes, can account for that degree of disparity.13 Schroeder and Dighiero suspected that CLL might be a heterogeneous disorder, but were unable to cull from the literature the comprehensive clinical detail needed to establish this. They did report, however, that some of the cases with mutated VH genes were CD5 negative and therefore not cases of classical CLL.
More recently, a multicenter study of 64 patients with surface IgM+, CD5+ CLL also found 2 groups of roughly equal numbers with respectively mutated and unmutated VHgenes.14 Although no clinical detail was available otherwise to distinguish the 2 subsets, the investigators were able to confirm the observation of Schroeder and Dighiero that the presence or absence of somatic mutations was associated with the use of particular VH genes.
In 1997, our group examined the VH genes of 22 patients with classical B-cell CLL segregated according to karyotype. Tumors with trisomy 12 had unmutated VH genes, but those with 13q14 abnormalities detected by conventional cytogenetics had evidence of somatic mutations.15 Because it has been previously shown that CLL patients with trisomy 12 have a poorer survival than those with abnormalities at 13q14,16 this pointed to an association between clinical status and degree of somatic mutation.
The suspicion that the clinical heterogeneity of CLL might have a biological basis led us to extend this study. We have now examined the Ig VH gene sequences in a series of 84 patients with classical B-cell CLL attending our hematology clinic and compared our results with various clinical characteristics of the patients and their survival. The striking finding to emerge is that the presence of VH gene mutations places the CLL patient in a disease group with a clearly better prognosis.
MATERIALS AND METHODS
Patients.
Patients were selected for study from over 600 cases of CLL who have attended our hematology clinic in recent years. An attempt was made to include a representative selection of karyotypic disorders, but most patients were chosen simply because they happened to be attending the outpatient clinic for routine follow-up. Twenty-two of the patients were included in the series linking trisomy 12 with the absence of somatic mutation that we reported recently.15 Almost all of the patients studied came from the local area and included many whose diagnosis was made incidentally from a blood count ordered for another purpose and whose CLL has remained entirely asymptomatic. It has been our practice, nevertheless, to continue to observe such asymptomatic patients once or twice a year. They were staged at diagnosis according to the Binet Classification.17 Immunophenotyping was performed afresh during the course of the current investigation. All cases scored 4 or 5 according to the Royal Marsden scoring system for CLL,1 were CD23 and CD5 positive, and had monotypic expression of weak surface Ig.
All patients have been followed for at least a year since diagnosis, the longest follow-up being 25 years. Patients were designated as having stable or progressive disease on the basis of the following criteria: lymphocyte count doubling time of less than 1 year; progression to a more advanced Binet stage; development of systemic symptoms; development of Richter’s syndrome; downward trend of hemoglobin (Hb) or platelet count to below the normal range (Hb < 13.5 g/dL for males and < 11.5 g/dL for females; platelet count < 150 × 109/L) even when not meeting the criteria for stage C disease (Hb < 10 g/dL; platelet count < 100 × 109/L). Possession of one of these characteristics was sufficient to qualify as progressive disease. Patients with progressive disease have generally been treated conventionally with chlorambucil as first line therapy and with fludarabine for those with resistant disease. Patients with stable disease were not offered chemotherapy.
Lymphocyte morphology was assessed on blood films stained with Jenner Geimsa. Atypical morphology was defined according to the criteria of Matutes et al18 as greater than 10% prolymphocytes or greater than 15% cells with cleaved nuclei and/or lymphoplasmacytoid cells in the blood of patients whose predominant cell type was a small lymphocyte with coarsely clumped chromatin.
Cytogenetics.
Whole peripheral blood was cultured at 37°C in the presence of tetradecanoyl phorbol 12-myristate 13-acetate (TPA) (0.05 μg/mL) for 3 to 5 days. Cells were treated with colcemid (0.1 μg/mL) for 60 minutes at 37°C before harvesting. After hypotonic treatment (KCL 0.075 mol/L for 10 minutes at 37°C), cells were resuspended in fixative (methanol: glacial acetic acid 3:1). Standard cytogenetic preparations were made, G banded, and karyotyped according to the International System for Cytogenetic Nomenclature (1995).
Preparation of cDNA and DNA.
Blood samples for testing were taken during the past 5 years. Some were tested immediately, while for others, the lymphocytes were cryopreserved and tested later. Because the VH gene signature is believed not to change during the clinical course of CLL, it was deemed satisfactory to determine this at any stage of the disease whether treated or not. The preferred source material was RNA, as this reduces the possibility of amplifying an aberrantly rearranged VH gene; cDNA was synthesized by reverse transcription using an oligo(dT) primer as previously described.19 Where RNA was not available, genomic DNA was extracted using the QIAmp blood kit (Qiagen, Hilden, Germany).
Amplification of VH genes.
One fifth to one third of a sample of cDNA was amplified by polymerase chain reaction (PCR) using a mixture of oligonucleotide 5′ primers specific for each leader sequence of the VH1 to VH6 families,20 together with either mixed 3′ primers complementary to the germ line JHregions21 or 3′ primers complementary to the constant region.14 When there was failure to amplify, an alternative mixture of 5′ primers specific for framework 1 region of VH1 to VH6 was substituted.21 In our hands, the VH1 leader primer also amplifies sequences from the closely related VH7 family. In all cases, PCR was performed in a final volume of 50 μL with 20 pmol of each primer, 50 μmol deoxyribonucleotide triphosphates (dNTPs), and 2.5 U Taq DNA polymerase with reaction buffer (Boehringer, Lewes, E Sussex, UK). Amplification consisted of an initial denaturation step of 3 minutes at 94°C followed by 30 cycles of 94°C, 56°C and 72°C for 45 seconds each, with a final extension step of 10 minutes at 72°C. All PCR reactions were performed in duplicate. For each PCR, a control with no added template was used to check for contamination.
Sequencing and cloning of PCR products.
Clonal sequences were determined by sequencing amplicons from at least 2 independent PCR reactions. The majority of samples were sequenced directly using an automated DNA sequencer (Applied Biosystems, Foster City, CA). However, for the first 35 cases, cloning of gel-purified products into pGEM-TA vector was performed.19,21 After transformation of JM109 competent cells, clones found to contain an insert of appropriate size by restriction analysis of plasmid DNA were sequenced.19 21 A minimum of 5 bacterial colonies were analyzed. In addition, in 3 later cases, direct sequencing was unsuccessful and the sequence was determined by cloning.
Analysis of Ig gene sequences.
Nucleotide sequences were aligned to EMBL/GenBank and current databases (V-BASE sequence directory,22 using MacVector 4.0 sequence analysis software; International Biotechnologies Inc, New Haven, CT). Where there was >2% deviation from a germline VHsequence, the Chang and Casali formula23 was used to determine whether the replacement mutations had undergone antigenic selection. We have followed the criteria of Corbett at al24in assigning membership of the 2 longer D gene families (D2 and D3), but the requirement for 10 consecutive nucleotides of identity are probably too stringent for the shorter D gene families, and we have followed Fais et al14 in requiring only 7 consecutive nucleotides with no more than 2 differences. We have eliminated DIR segments and “minor” D segments from analysis.24
Statistical analysis.
The significance of associations between characteristics was determined using Fisher’s exact test. Survival curves from date of diagnosis were plotted using GraphPad Prism (version 2) software (San Diego, CA). This program calculates survival fractions using the Kaplan-Meier method and compares survival curves using the log-rank test.
RESULTS
Clinical and cytogenetic features of patients studied.
We studied 35 women and 49 men with classical B-cell CLL. The mean age at diagnosis was 63.3 years (median, 65; range, 33 to 92). A total of 62 were stage A, 9 stage B, and 13 stage C. A total of 34 had progressive disease and 50 stable disease. Lymphocyte morphology was typical in 58 cases and atypical in 26 cases.
Karyotypes are shown in Tables 1 and2. Trisomy 12 was found as a single abnormality in 11 patients and in combination with other abnormalities in a further 15 patients. Nine patients had translocations or deletions at 13q14 as single abnormalities, and 7 had these in association with other abnormalities. Ten had translocations involving chromosomal regions close to Ig genes on chromosomes 14 and 22, mainly in association with other abnormalities. Deletions involving 11q23 were found in 8 patients. Twenty-three patients had a normal karyotype. In 2 patients, chromosomal analysis was not attempted, and in 2, no metaphases were obtained.
Use of VH, D, and JH genes.
In common with several other series,9,12,14 we found an overuse of the V1-69 gene. Twenty-eight of the 51 translatable VH genes were used in this series. Six genes accounted for 57% of cases. V1-69, V3-23, and V4-34 were each used on 10 occasions (each 11.9%) and V1-02, V3-30.3, and V3-07 were each used on 6 occasions (each 7.1%). However, the normal antibody repertoire does not use VH genes randomly, and V3-23 (13.9%), V3-07 (5.6%), and V3-30.3 (8.3%) are the VH genes most commonly used by normal CD5+ B cells.25 In addition, we have previously shown that the V4-34 gene product is used by between 2.9% to 10.8% of normal B cells.26 On the other hand, V1-69 is used by only 1.6% of normal B cells27 and therefore appears overrepresented in this series.
The majority of the tumors used JH4 (35 of 84; 41.7%) or JH6 (27 of 84; 37.1%), which is similar to their use in normal CD5+ B cells (52% and 27%, respectively).25
Because of extensive mutations or N additions or nucleotide loss, a D segment gene could not be assigned to the sequences in 31 cases. The most commonly used gene was D3-3 (DXP4), which was used in 8 cases, all of which had unmutated VH genes. In all, 17 of the 27 different D-segment genes were used. D segments were not used preferentially with any VH or JH gene, but could not be assigned in the cases with the greatest numbers of somatic mutations.
Somatic mutations.
Whereas the leukemic cells of 38 patients (45.2%) had VHgenes with ≥ 98% sequence homology with the nearest germline gene, the remaining 46 cases (54.8%) showed evidence of somatic hypermutation, dividing the series into 2 subsets.
There are clear differences between the 2 subsets. Patients with unmutated VH genes (Table 1) had characteristics associated with a more malignant type of disease than those with evidence of somatic mutations (Table 2). Those lacking mutations were significantly more likely to have advanced stage disease, whereas those with mutations were more likely to have stage A disease (P = .0009). Lack of mutations was significantly associated with progressive disease and the presence of mutations with stable disease (P < .0001). Atypical morphology was similarly associated with lack of mutations and typical morphology with their presence (P < .0001). Trisomy 12, as an isolated karyotypic abnormality, was significantly associated with a lack of somatic mutations (P = .0019), and deletions or translocations at 13q14 were significantly associated with their presence (P = .023).
There was a significant tendency for VH1 family genes (P = .0142) and especially V1-69 (P = .0038) to be used by the subset that lacked mutations. A similar tendency towards the use of the D3-3 gene segment was found in this subset (P = .0058), although there was no tendency for these gene segments to be used together.
For patients with unmutated VH genes, the mean age at diagnosis was 64.9 years (median, 66; range, 36 to 88). There were 13 women and 25 men. For patients with mutated VH genes, the mean age was slightly younger at 61.9 years (median, 63; range, 33 to 92), and the gender ratio was closer to unity with 22 women and 24 men, although these differences did not reach statistical significance.
Antigenic selection.
Analysis of the distribution of replacement and silent mutations23showed a clustering of replacement amino acids in CDR1 and CDR2 in 17 of 46 (37.0%) of the cases with somatic mutations and conservation of amino acid sequence in framework regions in 28 of 46 (60.9%).
Intraclonal heterogeneity.
In 38 cases, at least 5 separate clones were analyzed. No intraclonal heterogeneity was found. This is in contrast to the finding in follicular lymphoma and implies that cells showing somatic mutations were no longer under the influence of mutator enzymes and had therefore passed through the germinal center. In 3 cases, a second blood sample was analyzed respectively 5 years, 3 years, and 18 months after the first. In each case, the clonal sequence was identical with the original sequence (with respectively 0, 2, and 19 mutations).
Prognostic significance of VH gene mutations.
Survival curves were plotted according to the Kaplan-Meier method. Only 2 patients were censored as lost to follow-up. Graphs comparing the survival of patients with mutated and unmutated VH genes are plotted in Fig 1. The median survival for patients with unmutated VH genes was 117 months and for those with mutations, 293 months. The difference is very significant (P = .001). Because the unmutated group contains more patients with advanced stage disease, we plotted the survival curve for stage A patients only (Fig 2). Median survival was 95 months for the patients without mutations and 293 months for those with mutations. Again, the difference in survival was very significant (P = .0008).
DISCUSSION
Somatic mutation is believed to occur in germinal centers or similar structures.8 Thus, the presence of such mutations in over half of our cases of CLL and the statistical evidence supporting the occurrence of antigenic selection in some of the cases argues strongly that these are tumors of memory B cells and not of naı̈ve B cells.
In any study of CLL, it is important to establish that the series is not contaminated by other kinds of lymphoma. It is particularly important to exclude mantle cell lymphoma, which is also a tumor of CD5+ B cells and which has a much worse prognosis than CLL. Other diseases that must be excluded are splenic lymphoma with villous lymphocytes, of which a small proportion are reportedly CD5+,28 and follicular lymphoma in leukemic phase. In this series, we have tried very hard to exclude all such cases. All had a Royal Marsden score of 4 or 5. No case had t(11;14)(q13;q32) translocations. Although 7 had t(14;18)(q32;q21) or t(18;22)(q21;q11) translocations, it is important to stress that such structural abnormalities have been previously reported in CLL and are not confined to follicular lymphoma.29 None of these cases had cellular morphology or immunophenotype typical of follicular lymphoma, and none showed the intraclonal variation of immunoglobulin VH genes seen in that condition.30
Patients with unmutated VH genes had a distinctly more malignant disease and a much shorter survival than those with somatic mutations. They were more likely to have atypical morphology, advanced stage, and progressive disease. Such a distinct clinical course argues in favor of CLL comprising 2 separate types of tumor arising at different stages of B-cell maturation: 1 a pregerminal center naı̈ve B cell and 1 a postgerminal center memory B cell.
In this series of patients, the influence of karyotype on prognosis is less than in our previous report,15 perhaps because we have included here 5 patients with both trisomy 12 and abnormalities at 13q14. As more sensitive techniques such as fluorescent in situ hybridization and comparative genomic hybridization are applied, it is apparent that leukemic chromosomes are more complicated than has been appreciated using conventional cytogenetics. It is clear that much more detailed work is required to establish the influence of chromosomal abnormalities on the 2 types of CLL.
We confirm in this study the biased use of certain VH genes in CLL. Six genes accounted for over half of the cases. However, when Brezinschek et al25 analyzed the normal B-cell immunoglobulin repertoire by single cell PCR of DNA from B cells of 2 individuals, they found that many of the same genes were similarly overused. An exception is V1-69, which apparently not overused by normal B cells,27 yet has been reported consistently as the most commonly used VH gene in CLL, usually in unmutated form.9,14,31 V1-69 occurs in several polymorphic forms and there is variation in the number of copies of V1-69 between different individuals.32,33 It would be helpful, therefore, to investigate the normal use of VH genes from a wider range of normal individuals, including some from the same age range as patients with CLL, before concluding that this gene is used more commonly in CLL than in normals. Why the V1-69 gene is seen so commonly in CLL in unmutated form remains unanswered. None of our patients used the V4-39 gene, but this gene is also usually unmutated in the reports in the literature, even in cases expressing surface IgG.12,14 Explanations for these phenomena are available,14 but lack certainty at present.
The suggestion that there might be 2 types of CLL pursuing distinct clinical courses and definable by the stage of differentiation of the cell of origin is independently supported by the work of Damle et al.34 It raises many pathophysiological questions, but clinicians will be interested in the prognostic implications. Thirty-three of our 84 patients (39.3%) were diagnosed below the age of 60 and might today be considered as candidates for aggressive chemotherapy and stem cell autograft for this incurable disease. Knowledge that 19 of them belonged to a subtype with a median survival of 25 years and that the other 14 belonged to a subtype with a median survival of only 8 years would be valuable.
ACKNOWLEDGMENT
The authors acknowledge the help of Dr D. Zhu and A. Thompsett who performed some of the gene sequences. Professor G.T. Stevenson and Dr M. Glennie provided helpful discussions. Dr R. Chapman and Dr P. Thomas gave statistical advice.
Supported by a grant from Tenovus UK (T.J.H. and Z.D.).
The publication costs of this article were defrayed in part by page charge payment. This article must therefore be hereby marked “advertisement” in accordance with 18 U.S.C. section 1734 solely to indicate this fact.
REFERENCES
Author notes
Address reprint requests to Terry J. Hamblin, MD, Department of Haematology, Royal Bournemouth Hospital, Castle Lane East, Bournemouth BH7 7DW, Dorset, UK; e-mail terjoha@aol.com.