The CALR mutations enhance the expression of the immunosuppressive proteins GARP and LAP on peripheral blood lymphocytes through increased binding of activated platelets

Author:

Holmström Morten Orebo1ORCID,Ruders Josephine Hallundbæk1,Riley Caroline Hasselbalch2,Larsen Morten Kranker3ORCID,Grauslund Jacob Handlos1,Kjær Lasse3ORCID,Skov Vibe3ORCID,Ellervik Christina456,Guo Belinda B.7ORCID,Linden Matthew7,Hasselbalch Hans Carl3ORCID,Andersen Mads Hald18

Affiliation:

1. Department of Oncology, National Center for Cancer Immune Therapy Herlev University Hospital Herlev Denmark

2. Department of Haematology Rigshospitalet Copenhagen Denmark

3. Department of Haematology Zealand University Hospital Roskilde Denmark

4. Department of Clinical Biochemistry Zealand University Hospital Koege Denmark

5. Department of Laboratory Medicine Boston Children's Hospital, Harvard Medical School Boston Massachusetts USA

6. Department of Clinical Medicine, Faculty of Health and Medical Sciences University of Copenhagen Copenhagen Denmark

7. School of Biomedical Sciences University of Western Australia Crawley Western Australia Australia

8. Department of Immunology and Microbiology University of Copenhagen Copenhagen Denmark

Abstract

SummaryRecently, an antibody which inhibits the glycoprotein A repetitions predominant (GARP)‐mediated release of active transforming growth factor beta (TGFβ) from the TGFβ propeptide latency‐associated peptide (LAP) showed preclinical activity in a murine model of the chronic myeloproliferative neoplasms (MPN). Consequently, we investigated the expression of the immunosuppressive molecules LAP and GARP on peripheral blood lymphocytes from 56 MPN patients and 11 healthy donors (HD). We found that lymphocytes from patients with MPN express higher levels of LAP and GARP with no strong differences found between the different MPN diagnoses. The impact of clinical parameters on the expression of LAP and GARP by lymphocytes showed that patients with calreticulin (CALR)mut MPN have increased expression compared with HD and patients with the Januskinase2 (JAK2) mutation. The fraction of lymphocytes bound to activated platelets (aPLT) strongly correlate to LAP and GARP expression suggesting that it is not the lymphocytes themselves but aPLT, which confer the increased expression of GARP and LAP on MPN patient lymphocytes. Notably, no differences in neither platelet counts nor anti‐thrombotic therapy was identified between patients with JAK2‐ and CALRmut patients. Analysis of platelet gene expression failed to identify differences in expression of relevant genes between JAK2‐ and CALRmut patients.

Funder

Raine Medical Research Foundation

Cancer Council Western Australia

Novo Nordisk Fonden

Publisher

Wiley

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