Amino acid sequence homology of monoclonal serum free light chain dimers and tissue deposited light chains in AL amyloidosis: a pilot study

Author:

Goldis Rivka12,Kaplan Batia3,Arad Michael24,Dispenzieri Angela5,Dasari Surendra6,Kukuy Olga Lesya7,Simon Amos J.3,Dori Amir12,Shavit-Stein Efrat12,Ziv Tamar8,Murray David9,Kourelis Taxiarchis5,Gertz Morie A.5,Dominissini Dan21011,Magen Hila212,Muchtar Eli5

Affiliation:

1. Department of Neurology , Sheba Medical Center , Ramat Gan , Israel

2. Sackler Faculty of Medicine , Tel Aviv University , Tel Aviv , Israel

3. Institute of Hematology and Sheba Cancer Research Center, Sheba Medical Center , Ramat Gan , Israel

4. Heart Failure Institute, Leviev Heart Center, Sheba Medical Center , Ramat Gan , Israel

5. Division of Hematology , Mayo Clinic , Rochester , MN , USA

6. Department of Health Sciences Research , Mayo Clinic , Rochester , MN , USA

7. Institute of Nephrology and Hypertension, Sheba Medical Center , Ramat Gan , Israel

8. Smoler Protein Center, Faculty of Biology , Technion – Israel Institute of Technology , Haifa , Israel

9. Department of Laboratory Medicine and Pathology , Mayo Clinic , Rochester , MN , USA

10. The Genomics Unit, Sheba Cancer Research Center, Sheba Medical Center , Ramat Gan , Israel

11. Wohl Institute of Translational Medicine, Sheba Medical Center , Ramat Gan , Israel

12. Multiple Myeloma Unit, Hematology Department , Sheba Medical Center , Ramat Gan , Israel

Abstract

Abstract Objectives Diagnosis of light chain amyloidosis (AL) requires demonstration of amyloid deposits in a tissue biopsy followed by appropriate typing. Previous studies demonstrated increased dimerization of monoclonal serum free light chains (FLCs) as a pathological feature of AL. To further examine the pathogenicity of FLC, we aimed at testing amino acid sequence homology between circulating and deposited light chains (LCs). Methods Matched tissue biopsy and serum of 10 AL patients were subjected to tissue proteomic amyloid typing and nephelometric FLC assay, respectively. Serum FLC monomers (M) and dimers (D) were analyzed by Western blotting (WB) and mass spectrometry (MS). Results WB of serum FLCs showed predominance of either κ or λ type, in agreement with the nephelometric assay data. Abnormal FLC M–D patterns typical of AL amyloidosis were demonstrated in 8 AL-λ patients and in one of two AL-κ patients: increased levels of monoclonal FLC dimers, high D/M ratio values of involved FLCs, and high ratios of involved to uninvolved dimeric FLCs. MS of serum FLC dimers showed predominant constant domain sequences, in concordance with the tissue proteomic amyloid typing. Most importantly, variable domain sequence homology between circulating and deposited LC species was demonstrated, mainly in AL-λ cases. Conclusions This is the first study to demonstrate homology between circulating FLCs and tissue-deposited LCs in AL-λ amyloidosis. The applied methodology can facilitate studying the pathogenicity of circulating FLC dimers in AL amyloidosis. The study also highlights the potential of FLC monomer and dimer analysis as a non-invasive screening tool for this disease.

Publisher

Walter de Gruyter GmbH

Subject

Biochemistry (medical),Clinical Biochemistry,General Medicine

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