Enrichment-Free Single-Cell Detection and Morphogenomic Profiling of Myeloma Patient Samples to Delineate Circulating Rare Plasma Cell Clones

Ndacayisaba, Libere J.; Rappard, Kate; Shishido, Stephanie N.; Velasco, Carmen Ruiz; Matsumoto, Nicholas; Navarez, Rafael; Tang, Guilin; Lin, Pei; Setayesh, Sonia Maryam; Naghdloo, Amin; Hsu, Ching-Ju; Maney, Carlisle; Symer, David E.; Bethel, Kelly; Kelly, Kevin R.; Merchant, Akil; Orłowski, Robert Z.; Hicks, James; Mason, Jeremy; Manasanch, Elisabeth E.; Kühn, Peter

doi:10.3390/curroncol29050242

Cited by 4 publications

(16 citation statements)

References 58 publications

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“…The biomarker-based classified groups represented candidate PCs, committed clonotypic B cells, and plasmablasts ( Figure 3 A). Quantification of the different circulating rare cell groups across patients showed that CD138+ cells were more abundant in neoplastic myeloma and not in NDs, with a higher proportion being found in NDMM than in precursor states (SMM and MGUS) ( Figure 3 B–D), consistent with our prior observations [ 19 , 20 ]. BCMA+ cells were detected in all samples, including NDs, confirming that the expression of BCMA in early B cells, although suggested to be low, is detectable in our assay.…”

Section: Resultssupporting

confidence: 91%

“…Technical validation for CD138, CD45, and DAPI cells in HDSCAs has been previously reported [ 19 , 20 ]. In titration experiments with U266, MM.1S, and control Jurkat cells, BCMA expression was consistently higher in U266 and MM.1S across all concentration conditions, while no BCMA expression was detected in control Jurkat cells, as expected ( Figure S1A ).…”

Section: Resultsmentioning

confidence: 99%

“…The rationale for developing the BCMA assay is grounded in BCMA’s progressive expression across the B-cell differentiation spectrum ( Figure 1 A) and the increasing interest in this marker as a therapeutic target, as demonstrated by the rise in clinical studies over the past 9 years ( Figure 1 B). The selection criteria for CD138, CD45, and DAPI have been previously described in two validated myeloma assays for morphogenomic differentiation of malignant and normal PCs and identification of rare cell clones [ 19 , 20 ]. Here, we substituted CD56 with BCMA for a new immunofluorescence staining panel (CD138, BCMA, CD45, DAPI), with the primary goal of targeting key cells of interest ( Figure 1 C) and characterizing circulating B lymphocytes expressing BCMA in the PB of patients with PC neoplasms.…”

Section: Methodsmentioning

confidence: 99%

“…In this study, we report the technical development and initial genomic and clinical validation of a new slide-based, enrichment-free immunofluorescence assay (i.e., BCMA, CD138, CD45, DAPI) for the detection of circulating rare cells and morphogenomic profiling of BCMA+ cells in PC malignancies, hereafter referred to as the “BCMA assay”. The technical methodology is built on the established “no-cell-left-behind” approach of the high-definition single-cell assay (HDSCA) workflow—previously validated clinically for various pathologies, including breast cancer [ 14 ], myocardial infarction [ 15 ], melanoma [ 15 ], prostate cancer [ 16 ], bladder cancer [ 17 ], colorectal cancer [ 18 ], and multiple myeloma [ 19 , 20 ]—and has been optimized for the detection of BCMA expression for the characterization of MM precursor cells in PC neoplasia.…”

Section: Introductionmentioning

confidence: 99%

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Characterization of BCMA Expression in Circulating Rare Single Cells of Patients with Plasma Cell Neoplasms

Ndacayisaba

Rappard

Shishido

et al. 2022

IJMS

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B-cell maturation antigen (BCMA), a key regulator of B-cell proliferation and survival, is highly expressed in almost all cases of plasma cell neoplasms and B-lymphoproliferative malignancies. BCMA is a robust biomarker of plasma cells and a therapeutic target with substantial clinical significance. However, the expression of BCMA in circulating tumor cells of patients with hematological malignancies has not been validated for the detection of circulating plasma and B cells. The application of BCMA as a biomarker in single-cell detection and profiling of circulating tumor cells in patients’ blood could enable early disease profiling and therapy response monitoring. Here, we report the development and validation of a slide-based immunofluorescence assay (i.e., CD138, BCMA, CD45, DAPI) for enrichment-free detection, quantification, and morphogenomic characterization of BCMA-expressing cells in patients (N = 9) with plasma cell neoplasms. Varying morphological subtypes of circulating BCMA-expressing cells were detected across the CD138(+/−) and CD45(+/−) compartments, representing candidate clonotypic post-germinal center B cells, plasmablasts, and both normal and malignant plasma cells. Genomic analysis by single-cell sequencing and correlation to clinical FISH cytogenetics provides validation, with data showing that patients across the different neoplastic states carry both normal and altered BCMA-expressing cells. Furthermore, altered cells harbor cytogenetic events detected by clinical FISH. The reported enrichment-free liquid biopsy approach has potential applications as a single-cell methodology for the early detection of BCMA+ B-lymphoid malignancies and in monitoring therapy response for patients undergoing anti-BCMA treatments.

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Section: Resultssupporting

confidence: 91%

Section: Resultsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

See 2 more Smart Citations

Characterization of BCMA Expression in Circulating Rare Single Cells of Patients with Plasma Cell Neoplasms

Ndacayisaba

Rappard

Shishido

et al. 2022

IJMS

Self Cite

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“…In a different study, researchers used an enrichment-free four-plex immunofluorescence technique and single-cell DNA sequencing for identification and genomic classification of plasma cells to distinguish normal and malignant plasma cells in blood and BM aspirates from patients with newly diagnosed myeloma and monoclonal gammopathy of undetermined significance (MGUS) [ 33 ]. The results confirmed that peripheral blood plasma cells presented the same genomic modifications that were present in BM plasma cells.…”

Section: Liquid Biopsy and Circulating Tumour Cellsmentioning

confidence: 99%

Circulating Tumour Cells, Cell Free DNA and Tumour-Educated Platelets as Reliable Prognostic and Management Biomarkers for the Liquid Biopsy in Multiple Myeloma

Allegra

Cancemi

Mirabile

et al. 2022

Cancers

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Liquid biopsy is one of the fastest emerging fields in cancer evaluation. Circulating tumour cells and tumour-originated DNA in plasma have become the new targets for their possible employ in tumour diagnosis, and liquid biopsy can define tumour burden without invasive procedures. Multiple Myeloma, one of the most frequent hematologic tumors, has been the target of therapeutic progresses in the last few years. Bone marrow aspirate is the traditional tool for diagnosis, prognosis, and genetic evaluation in multiple myeloma patients. However, this painful procedure presents a relevant drawback for regular disease examination as it requires an invasive practice. Moreover, new data demonstrated that a sole bone marrow aspirate is incapable of expressing the multifaceted multiple myeloma genetic heterogeneity. In this review, we report the emerging usefulness of the assessment of circulating tumour cells, cell-free DNA, extracellular RNA, cell-free proteins, extracellular vesicles, and tumour-educated platelets to evaluate the changing mutational profile of multiple myeloma, as early markers of disease, reliable predictors of prognosis, and as useful tools to perform less invasive monitoring in multiple myeloma.

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Targeted single-cell proteomic analysis identifies new liquid biopsy biomarkers associated with multiple myeloma

Setayesh,

Ndacayisaba,

Rappard

et al. 2023

npj Precis. Onc.

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Multiple myeloma (MM) is accompanied by alterations to the normal plasma cell (PC) proteome, leading to changes to the tumor microenvironment and disease progression. There is a great need for understanding the consequences that lead to MM progression and for the discovery of new biomarkers that can aid clinical diagnostics and serve as targets for therapeutics. This study demonstrates the applicability of utilizing the single-cell high-definition liquid biopsy assay (HDSCA) and imaging mass cytometry to characterize the proteomic profile of myeloma. In our study, we analyzed ~87,000 cells from seven patient samples (bone marrow and peripheral blood) across the myeloma disease spectrum and utilized our multiplexed panel to characterize the expression of clinical markers for PC classification, additional potential therapeutic targets, and the tumor microenvironment cells. Our analysis showed BCMA, ICAM3 (CD50), CD221, and CS1 (SLAMF7) as the most abundantly expressed markers on PCs across all myeloma stages, with BCMA, ICAM3, and CD221 having significantly higher expression levels on disease versus precursor PCs. Additionally, we identify significantly elevated levels of expression for CD74, MUM1, CD229, CD44, IGLL5, Cyclin D1, UBA52, and CD317 on PCs from overt disease conditions compared to those from precursor states.

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Enrichment-Free Single-Cell Detection and Morphogenomic Profiling of Myeloma Patient Samples to Delineate Circulating Rare Plasma Cell Clones

Cited by 4 publications

References 58 publications

Characterization of BCMA Expression in Circulating Rare Single Cells of Patients with Plasma Cell Neoplasms

Characterization of BCMA Expression in Circulating Rare Single Cells of Patients with Plasma Cell Neoplasms

Circulating Tumour Cells, Cell Free DNA and Tumour-Educated Platelets as Reliable Prognostic and Management Biomarkers for the Liquid Biopsy in Multiple Myeloma

Targeted single-cell proteomic analysis identifies new liquid biopsy biomarkers associated with multiple myeloma

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