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Blood, Vol. 95 No. 12 (June 15), 2000:
pp. 3922-3928
NEOPLASIA
From the Departments of Dermatology and Pathology,
University of Graz, Austria; the Department of Dermatology,
University of Münster; the Department of Dermatology, University
of Munich; the Department of Dermatology, University of
Würzburg; and Dermatopathologisches Gemeinschaftslabor,
Friedrichshafen, Germany; and the Department of Dermatology,
Yale University, New Haven, CT.
Cutaneous B-cell infiltrates showing a prominent follicular growth
pattern with germinal centers are thought by some authors to represent
either marginal zone lymphomas with reactive germinal centers or
pseudolymphomas. To establish whether a true primary cutaneous
follicular lymphoma exists, we studied biopsies from 15 patients with
skin lesions characterized histopathologically by the presence of
B-cell infiltrates with follicular pattern. Staging investigations,
including bone marrow biopsy, were negative in all patients. All were
negative for bcl-2 protein expression and did not
present the t(14;18). In all biopsy specimens neoplastic follicles
showed 1 or more morphologic or immunophenotypic criteria of malignancy
(presence of a reduced mantle zone, absence of tingible body
macrophages, reduced proliferation rate). In 9 specimens a monoclonal
rearrangement of JH genes could be detected by polymerase chain reaction analysis. After laser beam microdissection, a band of
the same length could be observed in 6 probes from different follicles
from the same specimen, indicating the presence of the same monoclonal
population of follicle center cells. Follow-up examinations in all
patients revealed no evidence of extracutaneous spread (mean follow-up,
48.7 months). Our study demonstrates that primary cutaneous follicular
lymphoma represents a distinct entity of the cutaneous B-cell lymphomas.
(Blood. 2000;95:3922-3928)
In the classification for cutaneous lymphomas recently
published by the European Organization for Research and Treatment
of Cancer (EORTC)-Cutaneous Lymphoma Project Group, follicle center cell lymphoma (FCL) is considered the most common variant of the primary cutaneous B-cell lymphomas (PCBCL).1 This type of
PCBCL usually is evident histopathologically with a diffuse growth
pattern.2-7 The presence of a follicular pattern has been
reported only in a few patients.8 On the other hand, the
existence of a true cutaneous follicular lymphoma has been questioned
by some authors, who suggest that cases of cutaneous lymphoid
infiltrates showing a follicular pattern with prominent germinal
centers represent in fact either marginal zone lymphoma-immunocytoma
with reactive germinal centers or B-cell
pseudolymphoma.9-11 The main reason the existence of a
primary cutaneous follicular lymphoma is denied by these authors
resides in the negativity for bcl-2 protein expression and the
absence of the 14;18 interchromosomal translocation in these
cases.12-14 In contrast, both these features are observed in most follicular lymphomas of the lymph nodes.15-18
In this article we present 15 cases of cutaneous follicle center
lymphoma with prominent follicular growth pattern (follicle center
lymphoma, follicular). To establish the true nature of these lesions,
we analyzed clinicopathologic and molecular features of the infiltrates
by various techniques, including clonality analysis after laser beam
computerized microdissection.
Patients
Histology
Immunohistology Detailed immunophenotyping was performed for both groups on routinely fixed, paraffin-embedded tissue sections according to a previously described 3-step immunoperoxidase technique20 using a broad panel of monoclonal antibodies. Microwave enhancement was used for most of the antibodies. Second and third antibodies were obtained from Dakopatts (Glostrup, Denmark). Normal skin structures and tonsil tissues served as internal and external positive controls, respectively. Negative controls were performed by omitting the primary antibody or replacing it with normal human serum.Laser beam microdissection Laser beam microdissection was carried out in 12 patients with cutaneous follicular lymphoma, 3 patients with MZL, and 4 patients with B-cell pseudolymphoma. In all specimens analyzed, samples containing 60 to 100 cells each from at least 5 different follicles (or from all follicles if fewer than 5) and 5 different interfollicular areas from the same specimen were obtained for polymerase chain reaction (PCR) analysis. Microdissection was performed as follows: 4-µm sections cut from formalin-fixed, paraffin-embedded tissues were mounted on glass slides with a thickness of 0.17 mm (very thin glass slides are needed to prevent laser energy from being dispersed before reaching the section of tissue), deparaffinized, and stained with methyl green. An ultraviolet laser microscope system was then used to isolate particular populations of cells (UV-laser microbeam; PALM, Bernried, Germany). In short, a pulsed UV laser of high beam quality (nitrogen laser, wavelength 337 nm, maximum frequency 20 pulses/s, pulse duration 3 nsec) was combined with an inverse microscope and focused through an objective of high numerical aperture into the tissue plane. Beam spot diameter measured approximately 0.3 to 0.5 µm. Because of the extremely high energy density within the focal point (laser energy at object plane approximately 5 µJ), all biologic material is completely destroyed.21 Using the UV laser beam at a high repetition rate (approximately 20 pulses/s), a circle was cut around the target cells. This resulted in complete separation of the target population from neighboring tissues (Figure 1). For this procedure the laser beam was fixed while the section was carefully moved to perform the cutting desired. Microscopic movements of tissue sections were made possible by the use of a motorized, computer-driven stage of the microscope. With the aid of a motorized micromanipulator and a thin injection needle (single-use injection needle; diameter, 0.8 mm; Henke-Sass-Wolf GmbH, Tuttlingen, Germany), the isolated cells were scraped from the coverslip and placed in a proteinase K solution. The rate of successful collection of cells for DNA analysis with this method was more than 90%. The computer-controlled stage and the micromanipulator had the same high resolution of 40 nm per microstep. Travel speed varied from less than 1 µm to several mm per second.
Molecular biology Molecular analysis of the JH gene rearrangement was performed using a standard technique. Briefly, DNA was prepared from formalin-fixed, paraffin-embedded tissue specimens as described previously.22 The JH gene was analyzed using the semi-nested PCR technique described by Wan et al,23 with minor modifications. For the first PCR, 20 µg template DNA was used in a 50-µL PCR reaction containing dNTP (0.2 mmol/L), primers Fr3A and LJH (0.1 mmol/L each), MgCl2 (1 mmol/L), KCl (50 mmol/L), and Tris HCl, pH 8.3 (10 mmol/L). Thirty cycles of the reaction were carried out (denaturation, 94°C, 60 seconds; annealing, 57°C, 60 seconds; extension, 72°C, 60 seconds) followed by a 7-minute final extension step at 72°C. A second PCR was performed using 1 µL from the first PCR as template in 50 µL of the same buffer, but primer VLJH was used instead of LJH. Twenty-five cycles were carried out at the temperature setting of the first PCR.DNA sequencing For JH gene sequencing, amplified DNA fragments were separated on a 2.5% Metaphor agarose gel (FMC) and were purified using the QIAquick Gel Extraction Kit (Qiagen, Hilden, Germany). DNA preparation (60 ng) was submitted to a cycle sequencing reaction (ABI PRISM BigDye Terminator Cycle Sequencing Ready Reaction Kit; Perkin-Elmer-Cetus, Norwalk, CT) and was analyzed with the ABI PRISM 310 Genetic Analyzer (Perkin-Elmer-Cetus).
Clinical features Fifteen patients with follicular lymphoma (4 men, 11 women; mean age, 53.1 years; range, 24 to 87 years) had solitary (n = 4), clustered (n = 5), or multiple (n = 6) reddish plaques or tumors located on the scalp (n = 3), face (n = 4), trunk (n = 4), upper extremities (n = 1), or multiple sites (n = 3) (Figure 2, Table 1).
Histology All cases of follicular lymphoma were classified as grade 2 according to the REAL classification. Histology showed bottom-heavy lymphoid infiltrates with prominent follicular pattern (Figures 3 and 4). A well-formed mantle zone around most follicles was present only in 2 patients. In the other specimens the mantle zone was either reduced (11 patients) or nearly absent (2 patients) (Figure 5). A clear-cut marginal zone was never observed. Tingible body macrophages within follicles were present only in 1 patient and were absent in the other 14 patients. Cytomorphology of follicles in all patients showed variable proportions of centrocytes (cleaved follicle center cells) and centroblasts (Figure 6). The interfollicular areas revealed the presence of small lymphocytes and histiocytes admixed with a few larger cells and occasionally other inflammatory cells such as eosinophils and plasma cells.
Immunohistology In all patients with FCL, there was a predominant B-cell population (CD20+, CD79a+). Neoplastic follicles were outlined by CD21+ follicular dendritic cells. B-lymphocytes within follicles revealed CD20+, CD10+, CD5 , and CD43 phenotypes (Figure
7A). Scattered CD10+ large
B-lymphocytes also could be observed as solitary units or arranged in
small clusters in the interfollicular areas in 9 patients. Staining
with MIB-1 monoclonal antibody showed a decreased pattern of
proliferation activity of the follicles (defined as the presence of
less than 50% of positive cells) in 8 patients and a normal pattern in
the other 7 (Figure 7B). Follicle center cells showed a monoclonal
expression of  light chain in 1 patient and were negative for both
immunoglobulin light chains in the other 14 patients. Plasma cells,
when present, expressed light chains at a normal ratio. Staining for
the bcl-2 protein was negative in all follicles
but positive in mantle cells and in small T and B-lymphocytes within
interfollicular areas (Figure 7C). Variable numbers of reactive T
lymphocytes were present within the follicles and in the
interfollicular areas.
Molecular biology Analysis of the JH gene rearrangement after laser beam microdissection performed in 12 patients with FCL revealed in 6 of them the presence of a single band of the same length within samples from different follicles, indicating the existence of a monoclonal population of cells within different follicles from the same specimen (Figure 8A, Table 1). Interfollicular areas in these patients showed a polyclonal pattern of JH gene rearrangement, characterized by the presence of several bands of different lengths in the different areas analyzed. In 4 of the 6 patients showing the same distinct band within different follicles, a band of similar length could be detected also in 1 or more interfollicular areas from the same specimen, probably indicating the presence of neoplastic follicle center cells within these areas as well.
DNA sequencing Analysis of JH gene sequences was performed in 3 of the 6 patients with FCL showing a monoclonal population of follicle center cells by laser-based PCR. The same DNA sequences could be observed in samples from different follicles in all 3, confirming the monoclonality of follicle center cells. Neoplastic germinal center cells within interfollicular areas could be demonstrated by DNA sequencing in 1 of them.Treatment and follow-up Data on treatment and follow-up could be obtained for all patients (mean follow-up, 48.7 months; range, 11 to 113 months; median, 39 months) (Table 1). Extracutaneous spread was not observed. Recurrent disease developed in 4 of 5 patients treated by surgery alone; 2 of them are alive with skin disease after 21 and 31 months, respectively. After further therapy, complete remission resulted in 2 patients, and they are alive without disease after 38 and 113 months, respectively. The fifth patient is in complete remission after 14 months. Six patients treated by local radiotherapy achieved a complete response. Three of them are alive with no evidence of disease after 11, 39, and 81 months, respectively. The other 3 had recurrent lesions at the same locations or at different skin sites. After further radiotherapy, 2 of these 3 patients achieved complete remission and are alive without skin lesions after 79 and 95 months, respectively, whereas the third is alive with skin disease 13 months after first diagnosis. One patient achieved a partial response after local radiotherapy and is alive with disease 13 months after first diagnosis. Three patients treated with surgical excision followed by radiotherapy achieved complete remission. Two of them are alive with no evidence of disease after 63 and 65 months, respectively. The third patient had a cutaneous recurrence at the same location and is alive with skin disease 54 months after the first diagnosis.
B-cell lymphomas arising primary in the skin have been recognized recently as a distinct type of extranodal lymphoma with a particular clinicopathologic presentation and a favorable prognosis.1,25,26 Some authors maintain that they are neoplasms of germinal center cells, though a follicular pattern has been described only rarely27; others think that for the most part they represent examples of either immunocytoma or marginal zone lymphoma (MALT-type cutaneous lymphoma).9-11 We described herein 15 patients who had PCBCL with a clear-cut follicular growth pattern and demonstrated that these represent true examples of cutaneous follicular lymphoma.
We thank Uli Schmidbauer for preparing the excellent histologic sections and the immunohistochemical stainings.
Submitted August 23, 1999; accepted February 8, 2000.
Reprints: Lorenzo Cerroni, Department of Dermatology, University of Graz, Auenbruggerplatz 8, A-8036 Graz, Austria; e-mail: lorenzo.cerroni{at}kfunigraz.ac.at.
The publication costs of this article were defrayed in part by page charge payment. Therefore, and solely to indicate this fact, this article is hereby marked "advertisement" in accordance with 18 U.S.C. section 1734.
1.
Willemze R, Kerl H, Sterry W, et al.
EORTC classification for primary cutaneous lymphomas: a proposal from the cutaneous lymphoma study group of the European Organization for Research and Treatment of Cancer.
Blood.
1997;90:354 2. Willemze R, Meijer CJLM, Scheffer E, et al. Diffuse large cell lymphomas of follicular center cell origin presenting in the skin: a clinicopathologic and immunologic study of 16 patients. Am J Pathol. 1987;126:325[Abstract]. 3. Pimpinelli N, Santucci M, Bosi A, et al. Primary cutaneous follicular centre-cell lymphoma: a lymphoproliferative disease with favourable prognosis. Clin Exp Dermatol. 1989;14:12[Medline] [Order article via Infotrieve]. 4. Berti E, Gianotti R, Alessi E, Caputo R. Primary cutaneous follicular center cell lymphoma: immunophenotypical and immunogenotypical aspects. In: van Vloten WA,Willemze R,Lange Vejlsgaard G,Thomsen K, eds. Cutaneous Lymphomas and Pseudolymphomas. Basel: Karger.; 1990:196. 5. Berti E, Alessi E, Caputo R. Reticulohistiocytoma of the dorsum (morbus Crosti) and other B-cell lymphomas. Semin Diagn Pathol. 1991;8:82[Medline] [Order article via Infotrieve]. 6. Berti E, Alessi E, Caputo R, Gianotti R, Delia D, Vezzoni P. Reticulohistiocytoma of the dorsum. J Am Acad Dermatol. 1988;19:259[Medline] [Order article via Infotrieve]. 7. Kerl H, Kresbach H. Germinal center cell-derived lymphomas of the skin. J Dermatol Surg Oncol. 1984;10:291[Medline] [Order article via Infotrieve]. 8. Garcia CF, Weiss LM, Warnke RA, Wood GS. Cutaneous follicular lymphoma. Am J Surg Pathol. 1986;10:454[Medline] [Order article via Infotrieve]. 9. Slater DN. Are most primary cutaneous B-cell lymphomas `marginal cell lymphomas' [reply]? Br J Dermatol. 1995;133:953. 10. Slater DN. MALT and SALT: the clue to cutaneous B-cell lymphoproliferative disease. Br J Dermatol. 1994;131:557[Medline] [Order article via Infotrieve]. 11. Isaacson PG, Norton AJ. Extranodal lymphomas. New York: Churchill Livingstone; 1994. 12. Cerroni L, Volkenandt M, Rieger E, Soyer HP, Kerl H. bcl-2 protein expression and correlation with the interchromosomal 14;18 translocation in cutaneous lymphomas and pseudolymphomas. J Invest Dermatol. 1994;102:231[Medline] [Order article via Infotrieve].
13.
Delia D, Borrello MG, Berti E, et al.
Clonal immunoglobulin gene rearrangements and normal T-cell receptor, bcl-2, and c-myc genes in primary cutaneous B-cell lymphomas.
Cancer Res.
1989;49:4901 14. Triscott JA, Ritter JH, Swanson PE, Wick MR. Immunoreactivity for bcl-2 protein in cutaneous lymphomas and lymphoid hyperplasias. J Cutan Pathol. 1995;22:2[Medline] [Order article via Infotrieve].
15.
Hockenbery DM, Zutter M, Hickey W, Nahm M, Korsmeyer SJ.
bcl-2 protein is topographically restricted in tissues characterized by apoptotic cell death.
Proc Natl Acad Sci U S A.
1991;88:6961
16.
Tsujimoto Y, Cossman J, Jaffe E, Croce CM.
Involvement of the bcl-2 gene in human follicular lymphoma.
Science.
1985;228:1440 17. Gaulard P, D'Agay MF, Peuchmaur M, et al. Expression of the bcl-2 gene product in follicular lymphoma. Am J Pathol. 1992;140:1089[Abstract]. 18. Clark H, Jones DB, Jacobs P, Wright DH. Molecular and cytogenetic analysis of t(14;18) in nodal and extranodal lymphoma. J Pathol. 1990;161:340.
19.
Harris NL, Jaffe ES, Stein H, et al.
A revised European-American classification of lymphoid neoplasms: a proposal from the international lymphoma study group.
Blood.
1994;84:1361 20. Cerroni L, Smolle J, Soyer HP, Martinez Aparicio A, Kerl H. Immunophenotyping of cutaneous lymphoid infiltrates in frozen and paraffin-embedded tissue sections: a comparative study. J Am Acad Dermatol. 1990;22:405[Medline] [Order article via Infotrieve]. 21. Greulich KO, Leitz G. Light as microsensor and micromanipulator: laser microbeams and optical tweezers. Exp Technol Phys. 1994;40:1. 22. Popper HH, Winter E, Höfler G. DNA sequences of mycobacterium tuberculosis in formalin fixed and paraffin embedded tissue in tuberculosis and sarcoidosis detected by PCR. Am J Clin Pathol. 1994;101:738[Medline] [Order article via Infotrieve].
23.
Wan JH, Trainor KJ, Brisco MJ, Morley AA.
Monoclonality in B cell lymphoma detected in paraffin wax embedded sections using the polymerase chain reaction.
J Clin Pathol.
1990;43:888
24.
Gribben JG, Freedman AS, Woo SD, et al.
All advanced stage non-Hodgkin's lymphomas with a polymerase chain reaction amplifiable breakpoint of bcl-2 have residual cells containing the bcl-2 rearrangement at evaluation and after treatment.
Blood.
1991;78:3275 25. Santucci M, Pimpinelli N, Arganini L. Primary cutaneous B-cell lymphoma: a unique type of low-grade lymphoma: clinicopathologic and immunologic study of 83 cases. Cancer. 1991;67:2311[Medline] [Order article via Infotrieve]. 26. Cerroni L, Kerl H, Gatter K. An Illustrated Guide to Skin Lymphoma. London: Blackwell Science; 1998. 27. Willemze R, Rijlaarsdam JU, Meijer CJLM. Are most primary cutaneous B-cell lymphomas `marginal cell lymphomas'? Br J Dermatol. 1995;133:950[Medline] [Order article via Infotrieve]. 28. Isaacson PG. Malignant lymphomas with a follicular growth pattern. Histopathology. 1996;28:487[Medline] [Order article via Infotrieve]. 29. Nathwani BN, Winberg CD, Diamond LW, Bearman RM, Kim H. Morphologic criteria for the differentiation of follicular lymphoma from florid reactive follicular hyperplasia: a study of 80 cases. Cancer. 1981;48:1794[Medline] [Order article via Infotrieve]. 30. Ashton-Key M, Diss TC, Isaacson PG, Smith MEF. A comparative study of the value of immunohistochemistry and the polymerase chain reaction in the diagnosis of follicular lymphoma. Histopathology. 1995;27:501[Medline] [Order article via Infotrieve]. 31. Cerroni L, Minkus G, Pütz B, Höfler H, Kerl H. Laser beam microdissection in the diagnosis of cutaneous B-cell lymphoma. Br J Dermatol. 1997;136:743[Medline] [Order article via Infotrieve].
32.
Emmert-Buck MR, Bonner RF, Smith PD, et al.
Laser capture microdissection.
Science.
1996;274:998
33.
Dogan A, Du MQ, Aiello A, et al.
Follicular lymphomas contain a clonally linked but phenotypically distinct neoplastic B-cell population in the interfollicular zone.
Blood.
1998;91:4708 34. Mollejo M, Menarguez J, Cristobal E, et al. Monocytoid B cells: a comparative clinical pathologic study of their distribution in different types of low-grade lymphomas. Am J Surg Pathol. 1994;18:1131[Medline] [Order article via Infotrieve]. 35. Pileri S, Poggi S, Sabattini E, et al. Apoptosis as programmed cell death (PCD): Cupio dissolvi in cell life. Curr Diagn Pathol. 1994;1:48. 36. Pezzella F, Gatter KC, Mason DY, et al. bcl-2 Protein expression in follicular lymphomas in absence of 14;18 translocation. Lancet. 1990;336:1510[Medline] [Order article via Infotrieve]. 37. Ngan BY, Chen-Levy Z, Weiss LM, Warnke RA, Cleary ML. Expression in non-Hodgkin's lymphoma of the bcl-2 protein associated with the t(14;18) chromosomal translocation. N Engl J Med. 1988;318:1638[Abstract].
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  E. M. Buda-Okreglak, M. J. Walden, and M. D. Brissette Perineural CNS Invasion in Primary Cutaneous Follicular Center Lymphoma J. Clin. Oncol., October 10, 2007; 25(29): 4684 - 4686. [Full Text] [PDF]
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 O. K. Weinberg, W. Z. Ai, M. R. Mariappan, C. Shum, R. Levy, and D. A. Arber ''Minor'' BCL2 Breakpoints in Follicular Lymphoma: Frequency and Correlation with Grade and Disease Presentation in 236 Cases J. Mol. Diagn., September 1, 2007; 9(4): 530 - 537. [Abstract] [Full Text] [PDF]
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 L Cerroni Lymphoproliferative lesions of the skin. J. Clin. Pathol., August 1, 2006; 59(8): 813 - 826. [Abstract] [Full Text] [PDF]
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R. Dijkman, C. P. Tensen, E. S. Jordanova, J. Knijnenburg, J. J. Hoefnagel, A. A. Mulder, C. Rosenberg, A. K. Raap, R. Willemze, K. Szuhai, et al. Array-Based Comparative Genomic Hybridization Analysis Reveals Recurrent Chromosomal Alterations and Prognostic Parameters in Primary Cutaneous Large B-Cell Lymphoma J. Clin. Oncol., January 10, 2006; 24(2): 296 - 305. [Abstract] [Full Text] [PDF]
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Abstract
Introduction
positive). One
patient was negative for both 
