DETECTION OF MONOCLONALITY IN LOW-GRADE B-CELL LYMPHOMAS USING THE POLYMERASE CHAIN-REACTION IS DEPENDENT ON PRIMER SELECTION AND LYMPHOMA TYPE

被引：253

作者：

DISS, TC ^{[1
]}

PENG, HZ ^{[1
]}

WOTHERSPOON, AC ^{[1
]}

ISAACSON, PG ^{[1
]}

PAN, LX ^{[1
]}

机构：

[1] UNIV LONDON UNIV COLL,SCH MED,DEPT HISTOPATHOL,UNIV ST,LONDON WC1E 6JJ,ENGLAND

来源：

JOURNAL OF PATHOLOGY | 1993年 / 169卷 / 03期

关键词：

PCR; LOW-GRADE B-CELL LYMPHOMA; IMMUNOGLOBULIN HEAVY CHAIN GENE; MONOCLONALITY; FRAMEWORK-2; FRAMEWORK-3;

D O I：

10.1002/path.1711690303

中图分类号：

R73 [肿瘤学];

学科分类号：

100214 ;

摘要：

Detection of B-cell monoclonality using the polymerase chain reaction (PCR) promises the quick and cost-effective separation of monoclonal from polyclonal B-cell disease. However, the efficiency of the method has yet to be fully assessed, particularly with regard to disease type and selection of PCR primers. We have evaluated two approaches based on amplification of the immunoglobulin heavy chain gene using framework 2 (Fr2) and framework 3 (Fr3) region primers. Frozen tissue samples from 94 cases of low-grade B-cell lymphoma were investigated, all of which had previously been shown to be monoclonal by Southern blot analysis. Using a Fr2 primer, we were able to show monoclonality in 85 per cent of cases; with Fr3, 80 per cent of cases; and using both techniques in separate reactions, 90 per cent of cases. Thus, a significant false-negative rate exists with either primer which can be reduced by using both. We also found a difference in the efficiency of detection in different types of lymphoma; only 87 per cent of mucosa-associated lymphomas and centroblastic/centrocytic lymphomas were shown to be monoclonal, whereas all of the other lymphoma types tested were positive using one or both methods. We conclude that PCR detection of B-cell monoclonality allows rapid analysis of tissue samples, including paraffin-processed material. False-negative results which occur in some types of lymphoma can be reduced by the use of two or more primer combinations.

引用

页码：291 / 295

页数：5

共 17 条

[1] MANTLE CELL LYMPHOMA - A PROPOSAL FOR UNIFICATION OF MORPHOLOGICAL, IMMUNOLOGICAL, AND MOLECULAR-DATA [J].

BANKS, PM ;

CHAN, J ;

CLEARY, ML ;

DELSOL, G ;

DEWOLFPEETERS, C ;

GATTER, K ;

GROGAN, TM ;

HARRIS, NL ;

ISAACSON, PG ;

JAFFE, ES ;

MASON, D ;

PILERI, S ;

RALFKIAER, E ;

STEIN, H ;

WARNKE, RA .

AMERICAN JOURNAL OF SURGICAL PATHOLOGY, 1992, 16 (07) :637-640

[2] CLUSTERING OF EXTENSIVE SOMATIC MUTATIONS IN THE VARIABLE REGION OF AN IMMUNOGLOBULIN HEAVY-CHAIN GENE FROM A HUMAN B-CELL LYMPHOMA [J].

CLEARY, ML ;

MEEKER, TC ;

LEVY, S ;

LEE, E ;

TRELA, M ;

SKLAR, J ;

LEVY, R .

CELL, 1986, 44 (01) :97-106

[3] DETECTION OF IMMUNOGLOBULIN GENE REARRANGEMENT IN B-LYMPHOID MALIGNANCIES BY POLYMERASE CHAIN-REACTION GENE AMPLIFICATION [J].

DEANE, M ;

NORTON, JD .

BRITISH JOURNAL OF HAEMATOLOGY, 1990, 74 (03) :251-256

[4]

DEANE M, 1991, LEUKEMIA, V5, P726

[5]

Kabat E. A., 1987, SEQUENCES PROTEINS I, DOI 10.1016/0003-2697(84)90805-4

[6] SOMATIC MUTATION IN HUMAN B-CELL TUMORS [J].

LEVY, R ;

LEVY, S ;

CLEARY, ML ;

CARROLL, W ;

KON, S ;

BIRD, J ;

SKLAR, J .

IMMUNOLOGICAL REVIEWS, 1987, 96 :43-58

[7] RAPID METHOD FOR DISTINGUISHING CLONAL FROM POLYCLONAL B-CELL POPULATIONS IN SURGICAL BIOPSY SPECIMENS [J].

MCCARTHY, KP ;

SLOANE, JP ;

WIEDEMANN, LM .

JOURNAL OF CLINICAL PATHOLOGY, 1990, 43 (05) :429-432

[8]

MEEKER TC, 1988, J IMMUNOL, V141, P3994

[9] IMPROVED PCR METHOD FOR DETECTING MONOCLONAL IMMUNOGLOBULIN HEAVY-CHAIN REARRANGEMENT IN B-CELL NEOPLASMS [J].

RAMASAMY, I ;

BRISCO, M ;

MORLEY, A .

JOURNAL OF CLINICAL PATHOLOGY, 1992, 45 (09) :770-775

[10] SPLENIC MARGINAL ZONE CELL LYMPHOMA [J].

SCHMID, C ;

KIRKHAM, N ;

DISS, T ;

ISAACSON, PG .

AMERICAN JOURNAL OF SURGICAL PATHOLOGY, 1992, 16 (05) :455-466

← 1 2 →