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Literature DB >> 27927646

BCR-ABL-specific T-cell therapy in Ph+ ALL patients on tyrosine-kinase inhibitors.

Patrizia Comoli^1,2, Sabrina Basso^1,2, Giovanni Riva³, Patrizia Barozzi³, Ilaria Guido^1,2, Antonella Gurrado^1,2, Giuseppe Quartuccio^1,2, Laura Rubert¹, Ivana Lagreca³, Daniela Vallerini³, Fabio Forghieri³, Monica Morselli³, Paola Bresciani³, Angela Cuoghi³, Ambra Paolini³, Elisabetta Colaci³, Roberto Marasca³, Antonio Cuneo⁴, Lorenzo Iughetti⁵, Tommaso Trenti⁶, Franco Narni³, Robin Foà⁷, Marco Zecca¹, Mario Luppi³, Leonardo Potenza³.

Abstract

Although the emergence of bone marrow (BM)-resident p190BCR-ABL-specific T lymphocytes has been correlated with hematologic and cytogenetic remissions in patients with Philadelphia chromosome-positive acute lymphoblastic leukemia (Ph+ ALL) undergoing maintenance tyrosine-kinase inhibitor treatment, little is known about the possibility of culturing these cells ex vivo and using them in T-cell therapy strategies. We investigated the feasibility of expanding/priming p190BCR-ABL-specific T cells in vitro by stimulation with dendritic cells pulsed with p190BCR-ABL peptides derived from the BCR-ABL junctional region and alternative splicing, and of adoptively administering them to patients with relapsed disease. We report on the feasibility of producing clinical-grade BCR-ABL-specific cytotoxic T lymphocytes (CTLs), endowed with antileukemia activity, from Ph+ ALL patients and healthy donors. We treated 3 patients with Ph+ ALL with autologous or allogeneic p190BCR-ABL-specific CTLs. No postinfusion toxicity was observed, except for a grade II skin graft-versus-host disease in the patient treated for hematologic relapse. All patients achieved a molecular or hematologic complete remission (CR) after T-cell therapy, upon emergence of p190BCR-ABL-specific T cells in the BM. Our results show that p190BCR-ABL-specific CTLs are capable of controlling treatment-refractory Ph+ ALL in vivo, and support the development of adoptive immunotherapeutic approaches with BCR-ABL CTLs in Ph+ ALL.

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Year: 2016 PMID： 27927646 PMCID： PMC5290986 DOI： 10.1182/blood-2016-07-731091

Source DB: PubMed Journal: Blood ISSN： 0006-4971 Impact factor: 22.113

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