Analysis of monoclonal immunoglobulins from bone marrow plasma cells using immunopurification and LC-MS

Introduction: Clonal plasma cells secrete immunoglobulins, each with the exact same amino acid sequence, that are referred to as monoclonal immunoglobulins. The monoclonal heavy chain and light chain secreted from clonal plasma cells have the same molecular mass prior to the addition of post-transla...

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Main Authors: David R. Barnidge, Angela Dispenzieri, Dragan Jevremovic, David L. Murray
Format: Article
Language:English
Published: Elsevier 2023-04-01
Series:Journal of Mass Spectrometry and Advances in the Clinical Lab
Online Access:http://www.sciencedirect.com/science/article/pii/S2667145X23000226
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author David R. Barnidge
Angela Dispenzieri
Dragan Jevremovic
David L. Murray
author_facet David R. Barnidge
Angela Dispenzieri
Dragan Jevremovic
David L. Murray
author_sort David R. Barnidge
collection DOAJ
description Introduction: Clonal plasma cells secrete immunoglobulins, each with the exact same amino acid sequence, that are referred to as monoclonal immunoglobulins. The monoclonal heavy chain and light chain secreted from clonal plasma cells have the same molecular mass prior to the addition of post-translational modifications (PTMs) since their amino acid sequences are the same. Objective: To examine the molecular masses of monoclonal light chains and heavy chains isolated directly from the cytoplasm of bone marrow (BM) plasma cells and compare them to the serum derived monoclonal heavy and light chains. Methods: Using immunopurification and LC-MS we compared the molecular masses of immunoglobulins immunopurified from a patient’s serum to those immunopurified from the cytoplasm of their BM plasma cells. Results: Our findings demonstrate that the light chain molecular masses were identical whether they were obtained from serum or plasma cell cytoplasm. However, the heavy chain molecular masses did not match in bone marrow and serum due to differences in glycosylation, a common post-translational modification (PTM) found on the heavy chain. Conclusion: The data presented here show that by using LC-MS to analyze monoclonal immunoglobulins (also referred to as miRAMM) additional phenotype information is obtained at the cellular level which is complementary to other more common techniques such as flow cytometry and histopathology.
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spelling doaj.art-2a376106d54d4917ad3d93853460e73f2023-05-11T04:25:03ZengElsevierJournal of Mass Spectrometry and Advances in the Clinical Lab2667-145X2023-04-0128133141Analysis of monoclonal immunoglobulins from bone marrow plasma cells using immunopurification and LC-MSDavid R. Barnidge0Angela Dispenzieri1Dragan Jevremovic2David L. Murray3The Binding Site, Inc, Rochester, MN 55901, USADepartment of Laboratory Medicine and Pathology, Mayo Clinic Rochester, MN 55905, USA; Department of Medicine, Mayo Clinic, Rochester, MN 55905, USADepartment of Laboratory Medicine and Pathology, Mayo Clinic Rochester, MN 55905, USADepartment of Laboratory Medicine and Pathology, Mayo Clinic Rochester, MN 55905, USA; Corresponding author.Introduction: Clonal plasma cells secrete immunoglobulins, each with the exact same amino acid sequence, that are referred to as monoclonal immunoglobulins. The monoclonal heavy chain and light chain secreted from clonal plasma cells have the same molecular mass prior to the addition of post-translational modifications (PTMs) since their amino acid sequences are the same. Objective: To examine the molecular masses of monoclonal light chains and heavy chains isolated directly from the cytoplasm of bone marrow (BM) plasma cells and compare them to the serum derived monoclonal heavy and light chains. Methods: Using immunopurification and LC-MS we compared the molecular masses of immunoglobulins immunopurified from a patient’s serum to those immunopurified from the cytoplasm of their BM plasma cells. Results: Our findings demonstrate that the light chain molecular masses were identical whether they were obtained from serum or plasma cell cytoplasm. However, the heavy chain molecular masses did not match in bone marrow and serum due to differences in glycosylation, a common post-translational modification (PTM) found on the heavy chain. Conclusion: The data presented here show that by using LC-MS to analyze monoclonal immunoglobulins (also referred to as miRAMM) additional phenotype information is obtained at the cellular level which is complementary to other more common techniques such as flow cytometry and histopathology.http://www.sciencedirect.com/science/article/pii/S2667145X23000226
spellingShingle David R. Barnidge
Angela Dispenzieri
Dragan Jevremovic
David L. Murray
Analysis of monoclonal immunoglobulins from bone marrow plasma cells using immunopurification and LC-MS
Journal of Mass Spectrometry and Advances in the Clinical Lab
title Analysis of monoclonal immunoglobulins from bone marrow plasma cells using immunopurification and LC-MS
title_full Analysis of monoclonal immunoglobulins from bone marrow plasma cells using immunopurification and LC-MS
title_fullStr Analysis of monoclonal immunoglobulins from bone marrow plasma cells using immunopurification and LC-MS
title_full_unstemmed Analysis of monoclonal immunoglobulins from bone marrow plasma cells using immunopurification and LC-MS
title_short Analysis of monoclonal immunoglobulins from bone marrow plasma cells using immunopurification and LC-MS
title_sort analysis of monoclonal immunoglobulins from bone marrow plasma cells using immunopurification and lc ms
url http://www.sciencedirect.com/science/article/pii/S2667145X23000226
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