Selective targeting of multiple myeloma cells with a monoclonal antibody recognizing the ubiquitous protein CD98 heavy chain

表位 多发性骨髓瘤 单克隆抗体 免疫球蛋白轻链 抗体 分子生物学 造血 单克隆 抗原 化学 细胞生物学 癌症研究 生物 免疫学 干细胞
作者
Kana Hasegawa,Shunya Ikeda,Moto Yaga,Kouki Watanabe,Rika Urakawa,Akie Iehara,Mai Iwai,Seishin Hashiguchi,Soyoko Morimoto,Fumihiro Fujiki,Hiroko Nakajima,Jun Nakata,Sumiyuki Nishida,Akihiro Tsuboi,Yoshitaka Oka,Satoshi Yoshihara,Masahiro Manabe,Hiroyoshi Ichihara,Atsuko Mugitani,Yasutaka Aoyama
出处
期刊:Science Translational Medicine [American Association for the Advancement of Science]
卷期号:14 (632): eaax7706-eaax7706 被引量:35
标识
DOI:10.1126/scitranslmed.aax7706
摘要

Cancer-specific cell surface antigens are ideal therapeutic targets for monoclonal antibody (mAb)–based therapy. Here, we report that multiple myeloma (MM), an incurable hematological malignancy, can be specifically targeted by an mAb that recognizes a ubiquitously present protein, CD98 heavy chain (hc) (also known as SLC3A2). We screened more than 10,000 mAb clones raised against MM cells and identified R8H283, an mAb that bound MM cells but not normal hematopoietic or nonhematopoietic cells. R8H283 specifically recognized CD98hc. R8H283 did not react with monomers of CD98hc; instead, it bound CD98hc in heterodimers with a CD98 light chain (CD98lc), a complex that functions as an amino acid transporter. CD98 heterodimers were abundant on MM cells and took up amino acids for constitutive production of immunoglobulin. Although CD98 heterodimers were also present on normal leukocytes, R8H283 did not react with them. The glycoforms of CD98hc present on normal leukocytes were distinct from those present on MM cells, which may explain the lack of R8H283 reactivity to normal leukocytes. R8H283 exerted anti-MM effects without damaging normal hematopoietic cells. These findings suggested that R8H283 is a candidate for mAb-based therapies for MM. In addition, our findings showed that a cancer-specific conformational epitope in a ubiquitous protein, which cannot be identified by transcriptome or proteome analyses, can be found by extensive screening of primary human tumor samples.
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