High prevalence of the MYD88 mutation in testicular lymphoma: Immunohistochemical and genetic analyses

The activating mutation of MYD88 has been identified in diffuse large B‐cell lymphoma (DLBCL). We investigated the mutational status and both the gene amplification and protein expression of MYD88 in 23 cases of testicular DLBCL. To detect the MYD88 mutations, we employed the allele‐specific PCR and...

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Bibliographic Details
Published in:Pathology international 2015-10, Vol.65 (10), p.528-535
Main Authors: Oishi, Naoki, Kondo, Tetsuo, Nakazawa, Tadao, Mochizuki, Kunio, Tanioka, Fumihiko, Oyama, Toshio, Yamamoto, Tomoko, Iizuka, Junpei, Tanabe, Kazunari, Shibata, Noriyuki, Kirito, Keita, Katoh, Ryohei
Format: Article
Language:English
Subjects:
Adult
Aged
Aged, 80 and over
B-Lymphocytes - pathology
diffuse large B-cell lymphoma
gene amplification
Genetic Predisposition to Disease
Genetic Testing - methods
Humans
immunohistochemistry
Immunohistochemistry - methods
Lymphoma, Large B-Cell, Diffuse - epidemiology
Lymphoma, Large B-Cell, Diffuse - genetics
Lymphoma, Large B-Cell, Diffuse - pathology
Male
Middle Aged
mutation
Mutation - genetics
MYD88
Myeloid Differentiation Factor 88 - genetics
Prevalence
Testicular Neoplasms - epidemiology
Testicular Neoplasms - genetics
Testicular Neoplasms - pathology
testis
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Summary:The activating mutation of MYD88 has been identified in diffuse large B‐cell lymphoma (DLBCL). We investigated the mutational status and both the gene amplification and protein expression of MYD88 in 23 cases of testicular DLBCL. To detect the MYD88 mutations, we employed the allele‐specific PCR and Sanger sequencing. MYD88 gene amplification and protein expression were analyzed by quantitative PCR and by immunohistochemistry, respectively. There were 17 cases of primary testicular DLBCL: 94% (16/17) exhibited a non‐Germinal center B‐cell (non‐GCB) subtype, 82% (14/17) showed the MYD88 L265P, and 65% (11/17) had intense expression of MYD88. When compared with normal lymph nodes, the MYD88 is significantly amplified in primary testicular DLBCL. However, the amplification status showed no correlation with its mutational status or protein expression. Moreover, neither the MYD88 mutational status nor the expression pattern affected overall survival. Six cases were secondary testicular DLBCL with an 83% (5/6) and an 80% (4/5) incidence of the non‐GCB subtype and of the MYD88 L265P, respectively. In conclusion, we demonstrated a high prevalence of the non‐GCB subtype and the common MYD88 L265P in both primary and secondary testicular DLBCL. Our data suggest that the MYD88 mutation is a fairly consistent genetic feature in testicular DLBCL.
ISSN:1320-5463
1440-1827
DOI:10.1111/pin.12336