Transcriptional profiling of circulating tumor cells in multiple myeloma: a new model to understand disease dissemination

Garcés, Juan-José; Šimíček, Michal; Vicari, Marco; Brožová, Lucie; Burgos, Leire; Bezděková, Renata; Alignani, Diego; Calasanz, Marı́a José; Growková, Kateřina; Goicoechea, Ibai; Agirre, Xabier; Pour, Luděk; Prósper, Felipe; Ríos, Rafael; Martínez‐López, Joaquín; Millacoy, Pamela; Palomera, Luis; Orbe, Rafael Del; Perez-Montaña, Albert; Gárate, Sonia; Blanco, Laura; Lasa, Marta; Maiso, Patricia; Flores‐Montero, Juan; Sanoja-Flores, Luzalba; Chyra, Zuzana; Vdovin, Alexander; Ševčíková, Tereza; Jelı́nek, Tomáš; Botta, Cirino; Omri, Halima El; Keats, Jonathan J.; Órfão, Alberto; Hájek, Roman; Miguel, Jesús F. San; Paiva, Bruno

doi:10.1038/s41375-019-0588-4

Cited by 46 publications

(51 citation statements)

References 82 publications

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“…The early secretory cluster expressed both epithelial (EPCAM, KRT19) and mesenchymal (THY1, DCN) characteristics as well as smooth muscle actin and estrogen receptor, and thus bore some similarities to myoepithelial cells of the uterus. This population expresses IGFBP5 and LGALS1, genes implicated in homeostasis of stem and/or progenitor populations in normal and diseased tissues (Byrd et al, 2019;Garcés et al, 2020;Tumbar et al, 2004;You et al, 2018) and MEG3, an imprinted long noncoding RNA. Previous reports have identified an enrichment of stem cells in the fimbrial portion of the tube (Paik et al, 2012).…”

Section: Discussionmentioning

confidence: 99%

Single-cell Transcriptomics Identifies Gene Expression Networks Driving Differentiation and Tumorigenesis in the Human Fallopian Tube

Dinh

Lin

Abbasi

et al. 2020

Preprint

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The human fallopian tube harbors the cell-of-origin for the majority of high-grade serous 'ovarian' cancers (HGSCs), but its cellular composition, particularly the epithelial component, is poorly characterized. We performed single-cell transcriptomic profiling in 12 primary fallopian specimens from 8 patients, analyzing around 53,000 individual cells to map the major immune, fibroblastic and epithelial cell types present in this organ. We identified 10 epithelial sub-populations, characterized by diverse transcriptional programs including SOX17 (enriched in secretory epithelial cells), TTF3 and RFX3 (enriched in ciliated cells) and NR2F2 (enriched in early, partially differentiated secretory cells). Based on transcriptional signatures, we reconstructed a trajectory whereby secretory cells differentiate into ciliated cells via a RUNX3 high intermediate. Computational deconvolution of the cellular composition of advanced HGSCs based on epithelial subset signatures identified the 'early secretory' population as a likely precursor state for the majority of HGSCs. The signature of this rare population of cells comprised both epithelial (EPCAM, KRT) and mesenchymal (THY1, ACTA2) features, and was enriched in mesenchymal-type HGSCs (P = 6.7 x 10 -27 ), a group known to have particularly poor prognoses. This cellular and molecular compendium of the human fallopian tube in cancer-free women is expected to advance our understanding of the earliest stages of fallopian epithelial neoplasia.

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Section: Discussionmentioning

confidence: 99%

Single-cell Transcriptomics Identifies Gene Expression Networks Driving Differentiation and Tumorigenesis in the Human Fallopian Tube

Dinh

Lin

Abbasi

et al. 2020

Preprint

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“…Nonetheless, in one study, the frequency of CTPC in blood increased to 96% of newly-diagnosed MM patients when RNA was used instead of DNA to detect tumor IGH -V(D)J gene rearrangements [ 114 ]. However, to date, molecular analysis by next generation sequencing of blood-derived CTPC has preferentially focused on the molecular characterization of purified CTPC in order to better understand the biology of the disease [ 119 , 121 , 137 , 138 , 139 ]. In this regard, a recent study based on single-cell RNA sequencing reported that overexpression of CENPF and LGALS1 genes in CTPC from MM patients was associated with reduced progression free survival rates [ 119 ] ( Table 3 ).…”

Section: Detection Of Circulating Tumor Plasma Cellsmentioning

confidence: 99%

“…However, to date, molecular analysis by next generation sequencing of blood-derived CTPC has preferentially focused on the molecular characterization of purified CTPC in order to better understand the biology of the disease [ 119 , 121 , 137 , 138 , 139 ]. In this regard, a recent study based on single-cell RNA sequencing reported that overexpression of CENPF and LGALS1 genes in CTPC from MM patients was associated with reduced progression free survival rates [ 119 ] ( Table 3 ). In contrast, the clinical impact of next generation sequencing-based analysis of CTPC in MGUS, SMM and other plasma cell neoplasms currently remains unknown and deserves further investigation [ 137 ].…”

Section: Detection Of Circulating Tumor Plasma Cellsmentioning

confidence: 99%

“…For decades, the association observed between the presence (and greater numbers) of CTPC in blood and a higher tumor burden in the BM of MGUS, MM, PCL and other plasma cell neoplasms, has led to the notion that CTPC are a functionally unique population of BM-derived tumor PC [ 20 , 23 , 24 ]. However, more recent data indicates that CTPC usually represent a distinct subclone of BM PC [ 119 , 143 , 144 ] with a more immature phenotype ( Figure 3 ) and quiescent profile [ 21 , 144 , 145 ]. Thus, the association between blood and BM PC numbers could not be confirmed in several studies [ 20 , 118 , 129 ], or it has been shown to be a non-linear correlation [ 21 , 32 ] independent of sample quality (e.g., hemodilution).…”

Section: Biological Features and Physio-pathological Role Of Ctpc mentioning

confidence: 99%

“…From a genomic point of view, several studies have shown that (purified) CTPC (mostly) from MM patients reproduce the pattern of somatic mutations present in BM tumor PC with relatively high levels of (sub)clonal heterogeneity [ 137 , 143 ]. Thus, CTPC show overexpression of genes (and mutations/genetic alterations) associated with drug resistance [ 143 ], the inflammatory response (e.g., BIRC3 or TNFAIP 3), hypoxia (e.g., DDIT4 ), cell migration (e.g., CFAP54 , EZR , EMP3 or AHNAK ) and metastasis (e.g., AGR2 , DDX5 , MALAT1 , TMED2 , TPT1 ), together with downregulation of genes responsible for progression through the cell cycle (e.g., CENPF or CDC6 ) [ 119 ] ( Figure 4 A). In addition, the presence of CTPC in blood has also been related to ancestral cytogenetic profiles and unique cytogenetic alterations, including t(4;14) [ 28 , 29 , 116 ], deletion 13q [ 29 ], deletion 17p, t(11;14) and t(14;16) [ 22 ] ( Figure 4 B).…”

Section: Biological Features and Physio-pathological Role Of Ctpc mentioning

confidence: 99%

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Detection of Circulating Tumor Plasma Cells in Monoclonal Gammopathies: Methods, Pathogenic Role, and Clinical Implications

Sanoja-Flores

Flores‐Montero

Pérez-Andrés

et al. 2020

Cancers

Self Cite

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Cancer dissemination and distant metastasis most frequently require the release of tumor cells into the blood circulation, both in solid tumors and most hematological malignancies, including plasma cell neoplasms. However, detection of blood circulating tumor cells in solid tumors and some hematological malignancies, such as the majority of mature/peripheral B-cell lymphomas and monoclonal gammopathies, has long been a challenge due to their very low frequency. In recent years, the availability of highly-sensitive and standardized methods for the detection of circulating tumor plasma cells (CTPC) in monoclonal gammopathies, e.g., next-generation flow cytometry (NGF), demonstrated the systematic presence of CTPC in blood in virtually every smoldering (SMM) and symptomatic multiple myeloma (MM) patient studied at diagnosis, and in the majority of patients with newly-diagnosed monoclonal gammopathies of undetermined significance (MGUS). These methods set the basis for further detailed characterization of CTPC vs. their bone marrow counterpart in monoclonal gammopathies, to investigate their role in the biology of the disease, and to confirm their strong impact on patient outcome when measured both at diagnosis and after initiating therapy. Here, we review the currently available techniques for the detection of CTPC, and determine their biological features, physiopathological role and clinical significance in patients diagnosed with distinct diagnostic categories of plasma cell neoplasms.

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Investigating epithelial‐mesenchymal heterogeneity of tumors and circulating tumor cells with transcriptomic analysis and biophysical modeling

et al. 2021

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Cellular heterogeneity along the epithelial‐mesenchymal plasticity (EMP) spectrum is a paramount feature observed in tumors and circulating tumor cells (CTCs). High‐throughput techniques now offer unprecedented details on this variability at a single‐cell resolution. Yet, there is no current consensus about how EMP in tumors propagates to that in CTCs. To investigate the relationship between EMP‐associated heterogeneity of tumors and that of CTCs, we integrated transcriptomic analysis and biophysical modeling. We apply three epithelial‐mesenchymal transition (EMT) scoring metrics to multiple tumor samples and CTC datasets from several cancer types. Moreover, we develop a biophysical model that couples EMT‐associated phenotypic switching in a primary tumor with cell migration. Finally, we integrate EMT transcriptomic analysis and in silico modeling to evaluate the predictive power of several measurements of tumor aggressiveness, including tumor EMT score, CTC EMT score, fraction of CTC clusters found in circulation, and CTC cluster size distribution. Analysis of high‐throughput datasets reveals a pronounced heterogeneity without a well‐defined relation between EMT traits in tumors and CTCs. Moreover, mathematical modeling predicts different phases where CTCs can be less, equally, or more mesenchymal than primary tumor depending on the dynamics of phenotypic transition and cell migration. Consistently, various datasets of CTC cluster size distribution from different cancer types are fitted onto different regimes of the model. By further constraining the model with experimental measurements of tumor EMT score, CTC EMT score, and fraction of CTC cluster in bloodstream, we show that none of these assays alone can provide sufficient information to predict the other variables. In conclusion, we propose that the relationship between EMT progression in tumors and CTCs can be variable, and in general, predicting one from the other may not be as straightforward as tacitly assumed.

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Transcriptional profiling of circulating tumor cells in multiple myeloma: a new model to understand disease dissemination

Cited by 46 publications

References 82 publications

Single-cell Transcriptomics Identifies Gene Expression Networks Driving Differentiation and Tumorigenesis in the Human Fallopian Tube

Single-cell Transcriptomics Identifies Gene Expression Networks Driving Differentiation and Tumorigenesis in the Human Fallopian Tube

Detection of Circulating Tumor Plasma Cells in Monoclonal Gammopathies: Methods, Pathogenic Role, and Clinical Implications

Investigating epithelial‐mesenchymal heterogeneity of tumors and circulating tumor cells with transcriptomic analysis and biophysical modeling

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