Your search keyword '"Romay B"' showing total 11 results

1. [Evaluation of a multiplex PCR assay to differentiate mycobacteria of the Mycobacterium tuberculosis complex in a reference laboratory]

Author

Nailet, Arráiz R, Zolay, Romay B, and Nelba, Faría M

Subjects

DNA, Bacterial, Base Sequence, Molecular Sequence Data, Oligonucleotides, Humans, Tuberculosis, Mycobacterium tuberculosis, Mycobacterium bovis, Polymerase Chain Reaction, Genome, Bacterial, Bacterial Typing Techniques

Abstract

Mycobacteria that cause tuberculosis in animals and humans belong to the Mycobacterium tuberculosis complex. Techniques for conventional diagnosis are time-consuming and do not differentiate between different strains belonging to the M. tuberculosis complex. The aim of this study was to evaluate a multiplex PCR assay applicable to mycobacteria in culture with the capacity to differentiate different strains belonging to the M. tuberculosis complex in a reference laboratory. Primers based on genomics regions of difference (RD) consisting in DNA segments that are present in M. tuberculosis, but differentially deleted in several members of M. tuberculosis complex were used in a PCR assay. The test was applied to 86 clinical isolates of mycobacteria. The pattern of amplification allowed differentiating between M. tuberculosis, M. bovis and M. bovis BCG in a single PCR reaction. This PCR multiplex assay may be used in a Reference Laboratory of Tuberculosis Diagnosis as a complementary test to differentiate mycobacteria strains belonging to the M. tuberculosis complex. This test significantly reduces the time period between culture and strain identification, and thus for could favor the adoption of better strain specific antimycobacterial regimens as well as identification of zoonotic transmission of M. bovis to humans.

Published

2007

2. Evaluación de un ensayo de RPC múltiple para diferenciar micobacterias del complejo Mycobacterium tuberculosis en un laboratorio de referencia

Author

Arráiz R, Nailet, Romay B, Zolay, and Faría M, Nelba

Subjects

laboratorio de referencia, RD1, RPC múltiple, Mycobacterium tuberculosis complex, reference laboratory, multiplex PCR, Mycobacterium bovis, RD4, Complejo Mycobacterium tuberculosis

Abstract

Las micobacterias que causan tuberculosis en animales y humanos pertenecen al complejo Mycobacterium tuberculosis. Las técnicas de diagnóstico convencional, además de ser lentas y laboriosas, no permiten diferenciar entre miembros de este complejo. El objetivo de este estudio fue evaluar ensayos de RPC múltiple para contribuir a la identificación diferencial de micobacterias del complejo M. tuberculosis a partir de cultivos, en un laboratorio de referencia. Se utilizaron oligonucleótidos partidores basados en regiones de diferencia (RD) que consisten en segmentos de ADN que están presentes en M. tuberculosis, pero que han sido eliminados diferencialmente del genoma de otros miembros del complejo M. tuberculosis. El ensayo se aplicó sobre 86 aislados clínicos de micobacterias. El patrón de amplificación permitió diferenciar entre cepas de M. tuberculosis, M. bovis y M. bovis variedad BCG en una única RPC. Este ensayo de RPC múltiple puede ser utilizado en el Laboratorio de Referencia de Diagnóstico de Tuberculosis como prueba complementaria para diferenciar micobacterias del complejo M. tuberculosis, contribuyendo a un acortamiento en el período de reporte de resultados y un tratamiento adecuado del paciente, y podría ser aplicado también en estudios epidemiológicos de transmisión zoonótica de M. bovis a humanos Mycobacteria that cause tuberculosis in animals and humans belong to the Mycobacterium tuberculosis complex. Techniques for conventional diagnosis are time-consuming and do not differentiate between different strains belonging to the M. tuberculosis complex. The aim of this study was to evaluate a multiplex PCR assay applicable to mycobacteria in culture with the capacity to differentiate different strains belonging to the M. tuberculosis complex in a reference laboratory. Primers based on genomics regions of difference (RD) consisting in DNA segments that are present in M. tuberculosis, but differentially deleted in several members of M. tuberculosis complex were used in a PCR assay. The test was applied to 86 clinical isolates of mycobacteria. The pattern of amplification allowed differentiating between M. tuberculosis, M. bovis and M. bovis BCG in a single PCR reaction. This PCR multiplex assay may be used in a Reference Laboratory of Tuberculosis Diagnosis as a complementary test to differentiate mycobacteria strains belonging to the M. tuberculosis complex. This test significantly reduces the time period between culture and strain identification, and thus for could favor the adoption of better strain specific antimycobacterial regimens as well as identification of zoonotic transmission of M. bovis to humans

Published

2007

3. Evaluación de un ensayo de RPC múltiple para diferenciar micobacterias del complejo Mycobacterium tuberculosis en un laboratorio de referencia

Author

Zolay Romay B, Nelba Faría M, and Nailet Arráiz R

Subjects

laboratorio de referencia, Public Health, Environmental and Occupational Health, Biology, Reference laboratory, biology.organism_classification, Molecular biology, Mycobacterium bovis, Complejo Mycobacterium tuberculosis, Infectious Diseases, RD1, Mycobacterium tuberculosis complex, RPC múltiple, Multiplex polymerase chain reaction, RD4

Abstract

Las micobacterias que causan tuberculosis en animales y humanos pertenecen al complejo Mycobacterium tuberculosis. Las tecnicas de diagnostico convencional, ademas de ser lentas y laboriosas, no permiten diferenciar entre miembros de este complejo. El objetivo de este estudio fue evaluar ensayos de RPC multiple para contribuir a la identificacion diferencial de micobacterias del complejo M. tuberculosis a partir de cultivos, en un laboratorio de referencia. Se utilizaron oligonucleotidos partidores basados en regiones de diferencia (RD) que consisten en segmentos de ADN que estan presentes en M. tuberculosis, pero que han sido eliminados diferencialmente del genoma de otros miembros del complejo M. tuberculosis. El ensayo se aplico sobre 86 aislados clinicos de micobacterias. El patron de amplificacion permitio diferenciar entre cepas de M. tuberculosis, M. bovis y M. bovis variedad BCG en una unica RPC. Este ensayo de RPC multiple puede ser utilizado en el Laboratorio de Referencia de Diagnostico de Tuberculosis como prueba complementaria para diferenciar micobacterias del complejo M. tuberculosis, contribuyendo a un acortamiento en el periodo de reporte de resultados y un tratamiento adecuado del paciente, y podria ser aplicado tambien en estudios epidemiologicos de transmision zoonotica de M. bovis a humanos

Published

2007

4. Evaluación de un ensayo de RPC múltiple para diferenciar micobacterias del complejo Mycobacterium tuberculosis en un laboratorio de referencia

Author

Arráiz R, Nailet, primary, Romay B, Zolay, additional, and Faría M, Nelba, additional

Published

2007

5. Metabolic regulation of RA macrophages is distinct from RA fibroblasts and blockade of glycolysis alleviates inflammatory phenotype in both cell types.

Author

Umar S, Palasiewicz K, Volin MV, Romay B, Rahat R, Tetali C, Arami S, Guma M, Ascoli C, Sweiss N, Zomorrodi RK, O'Neill LAJ, and Shahrara S

Subjects

Animals, Antimetabolites pharmacology, Arthritis, Experimental physiopathology, Cell Movement, Cytokines, Fibroblasts drug effects, Fibroblasts metabolism, Fibroblasts pathology, Humans, Inflammation etiology, Inflammation metabolism, Inflammation pathology, Macrophages drug effects, Macrophages metabolism, Macrophages pathology, Mice, Mice, Inbred DBA, Pentose Phosphate Pathway, Phenotype, Arthritis, Rheumatoid physiopathology, Deoxyglucose pharmacology, Fibroblasts immunology, Glycolysis, Inflammation prevention & control, Macrophages immunology, Th17 Cells immunology

Abstract

Recent studies have shown the significance of metabolic reprogramming in immune and stromal cell function. Yet, the metabolic reconfiguration of RA macrophages (MΦs) is incompletely understood during active disease and in crosstalk with other cell types in experimental arthritis. This study elucidates a distinct regulation of glycolysis and oxidative phosphorylation in RA MΦs compared to fibroblast (FLS), although PPP (Pentose Phosphate pathway) is similarly reconfigured in both cell types. 2-DG treatment showed a more robust impact on impairing the RA M1 MΦ-mediated inflammatory phenotype than IACS-010759 (IACS, complexli), by reversing ERK, AKT and STAT1 signaling, IRF8/3 transcription and CCL2 or CCL5 secretion. This broader inhibitory effect of 2-DG therapy on RA M1 MΦs was linked to dysregulation of glycolysis (GLUT1, PFKFB3, LDHA, lactate) and oxidative PPP (NADP conversion to NADPH), while both compounds were ineffective on oxidative phosphorylation. Distinctly, in RA FLS, 2-DG and IACS therapies constrained LPS/IFNγ-induced AKT and JNK signaling, IRF5/7 and fibrokine expression. Disruption of RA FLS metabolic rewiring by 2-DG or IACS therapy was accompanied by a reduction of glycolysis (HIF1α, PFKFB3) and suppression of citrate or succinate buildup. We found that 2-DG therapy mitigated CIA pathology by intercepting joint F480 + iNOS + MΦ, Vimentin + fibroblast and CD3 + T cell trafficking along with downregulation of IRFs and glycolytic intermediates. Surprisingly, IACS treatment was inconsequential on CIA swelling, cell infiltration, M1 and Th1/Th17 cytokines (IFN-γ/IL-17) and joint glycolytic mediators. Collectively, our results indicate that blockade of glycolysis is more effective than inhibition of complex 1 in CIA, in part due to its effectiveness on the MΦ inflammatory phenotype., (© 2021. The Author(s), under exclusive licence to Springer Nature Switzerland AG.)

Published

2021

6. Interleukin-34 Reprograms Glycolytic and Osteoclastic Rheumatoid Arthritis Macrophages via Syndecan 1 and Macrophage Colony-Stimulating Factor Receptor.

Author

Van Raemdonck K, Umar S, Palasiewicz K, Volin MV, Elshabrawy HA, Romay B, Tetali C, Ahmed A, Amin MA, Zomorrodi RK, Sweiss N, and Shahrara S

Subjects

Animals, Glycolysis physiology, Inflammation metabolism, Mice, Osteoclasts metabolism, Phosphorylation, Synovial Membrane metabolism, Arthritis, Rheumatoid metabolism, Interleukins metabolism, Macrophages metabolism, Receptor, Macrophage Colony-Stimulating Factor metabolism, Syndecan-1 metabolism

Abstract

Objective: In rheumatoid arthritis (RA), elevated serum interleukin-34 (IL-34) levels are linked with increased disease severity. IL-34 binds to 2 receptors, macrophage colony-stimulating factor receptor (M-CSFR) and syndecan 1, which are coexpressed in RA macrophages. Expression of both IL-34 and syndecan 1 is strikingly elevated in the RA synovium, yet their mechanisms of action remain undefined. This study was undertaken to investigate the mechanism of action of IL-34 in RA., Methods: To characterize the significance of IL-34 in immunometabolism, its mechanism of action was elucidated in joint macrophages, fibroblasts, and T effector cells using RA and preclinical models., Results: Intriguingly, syndecan 1 activated IL-34-induced M-CSFR phosphorylation and reprogrammed RA naive cells into distinctive CD14+CD86+GLUT1+ M34 macrophages that expressed elevated levels of IL-1β, CXCL8, and CCL2. In murine M34 macrophages, the inflammatory phenotype was accompanied by potentiated glycolytic activity, exhibited by transcriptional up-regulation of GLUT1, c-Myc, and hypoxia-inducible factor 1α (HIF-1α) and amplified pyruvate and l-lactate secretion. Local expression of IL-34 provoked arthritis by expanding the glycolytic F4/80-positive, inducible nitric oxide synthase (iNOS)-positive macrophage population, which in turn attracted fibroblasts and polarized Th1/Th17 cells. The cross-talk between murine M34 macrophages and Th1/Th17 cells broadened the inflammatory and metabolic phenotypes, resulting in the expansion of IL-34 pathogenicity. Consequently, IL-34-instigated joint inflammation was alleviated in RAG -/- mice compared to wild-type mice. Syndecan 1 deficiency attenuated IL-34-induced arthritis by interfering with joint glycolytic M34 macrophage and osteoclast remodeling. Similarly, inhibition of glycolysis by 2-deoxy-d-glucose reversed the joint swelling and metabolic rewiring triggered by IL-34 via HIF-1α and c-Myc induction., Conclusion: IL-34 is a novel endogenous factor that remodels hypermetabolic M34 macrophages and facilitates their cross-regulation with T effector cells to advance inflammatory bone destruction in RA., (© 2021, American College of Rheumatology.)

Published

2021

7. IRAK4 inhibition: a promising strategy for treating RA joint inflammation and bone erosion.

Author

Umar S, Palasiewicz K, Van Raemdonck K, Volin MV, Romay B, Amin MA, Zomorrodi RK, Arami S, Gonzalez M, Rao V, Zanotti B, Fox DA, Sweiss N, and Shahrara S

Subjects

Animals, Fibroblasts metabolism, Humans, Inflammation metabolism, Interleukin-1 Receptor-Associated Kinases metabolism, Interleukin-12 metabolism, Tumor Necrosis Factor Inhibitors, Arthritis, Experimental metabolism, Arthritis, Rheumatoid

Abstract

Flares of joint inflammation and resistance to currently available biologic therapeutics in rheumatoid arthritis (RA) patients could reflect activation of innate immune mechanisms. Herein, we show that a TLR7 GU-rich endogenous ligand, miR-Let7b, potentiates synovitis by amplifying RA monocyte and fibroblast (FLS) trafficking. miR-Let7b ligation to TLR7 in macrophages (MΦs) and FLSs expanded the synovial inflammatory response. Moreover, secretion of M1 monokines triggered by miR-Let7b enhanced Th1/Th17 cell differentiation. We showed that IRAK4 inhibitor (i) therapy attenuated RA disease activity by blocking TLR7-induced M1 MΦ or FLS activation, as well as monokine-modulated Th1/Th17 cell polarization. IRAK4i therapy also disrupted RA osteoclastogenesis, which was amplified by miR-Let7b ligation to joint myeloid TLR7. Hence, the effectiveness of IRAK4i was compared with that of a TNF inhibitor (i) or anti-IL-6R treatment in collagen-induced arthritis (CIA) and miR-Let7b-mediated arthritis. We found that TNF or IL-6R blocking therapies mitigated CIA by reducing the infiltration of joint F480 + iNOS + MΦs, the expression of certain monokines, and Th1 cell differentiation. Unexpectedly, these biologic therapies were unable to alleviate miR-Let7b-induced arthritis. The superior efficacy of IRAK4i over anti-TNF or anti-IL-6R therapy in miR-Let7b-induced arthritis or CIA was due to the ability of IRAK4i therapy to restrain the migration of joint F480 + iNOS + MΦs, vimentin + fibroblasts, and CD3 + T cells, in addition to negating the expression of a wide range of monokines, including IL-12, MIP2, and IRF5 and Th1/Th17 lymphokines. In conclusion, IRAK4i therapy may provide a promising strategy for RA therapy by disconnecting critical links between inflammatory joint cells., (© 2020. CSI and USTC.)

Published

2021

8. Tofacitinib therapy intercepts macrophage metabolic reprogramming instigated by SARS-CoV-2 Spike protein.

Author

Palasiewicz K, Umar S, Romay B, Zomorrodi RK, and Shahrara S

Subjects

Arthritis, Rheumatoid metabolism, COVID-19 metabolism, Cells, Cultured, Fibroblasts drug effects, Fibroblasts metabolism, Humans, Interleukin-6 metabolism, Macrophages metabolism, Receptors, Interleukin-6 metabolism, STAT1 Transcription Factor metabolism, STAT3 Transcription Factor metabolism, Signal Transduction drug effects, Tumor Necrosis Factor-alpha metabolism, Macrophages drug effects, Piperidines pharmacology, Pyrimidines pharmacology, SARS-CoV-2 drug effects, Spike Glycoprotein, Coronavirus metabolism, COVID-19 Drug Treatment

Abstract

The molecular mechanism of severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) Spike protein was characterized to identify novel therapies. The impact of tofacitinib, IL-6R Ab, or TNFi therapy was determined on Spike protein or LPS/IFN-γ-induced signaling, inflammation, and metabolic reprogramming in MΦs and/or rheumatoid arthritis (RA) fibroblast-like synoviocyte (FLS). ACE2 frequency was markedly expanded in MΦs compared to T cells and RA FLS. Tofacitinib suppresses Spike protein potentiated STAT1 signaling, whereas this function was unchanged by TNFi. Tofacitinib impairs IL-6/IFN/LPS-induced STAT1 and STAT3 phosphorylation in RA MΦs and FLS. Interestingly, tofacitinib had a broader inhibitory effect on the monokines, glycolytic regulators, or oxidative metabolites compared to IL-6R Ab and TNFi in Spike-protein-activated MΦs. In contrast, all three therapies disrupted IFN-α and IFN-β secretion in response to Spike protein; nonetheless, the IFN-γ was only curtailed by tofacitinib or IL-6R Ab. While tofacitinib counteracted MΦ metabolic rewiring instigated by Spike protein, it was inconsequential on the glycolysis expansion mediated via HK2 and/or LDHA in the activated RA MΦ and FLS. Nevertheless, the potentiated inflammatory response and the diminished oxidative phosphorylation modulated by Spike protein and/or LPS/IFN-γ stimulation in MΦs or RA FLS were reversed by tofacitinib. In conclusion, tofacitinib suppresses MΦ inflammation and immunometabolism triggered by Spike protein and may provide a promising strategy for COVID-19 patients., (© 2021 Wiley-VCH GmbH.)

Published

2021

9. CCL25 and CCR9 is a unique pathway that potentiates pannus formation by remodeling RA macrophages into mature osteoclasts.

Author

Umar S, Palasiewicz K, Van Raemdonck K, Volin MV, Romay B, Ahmad I, Tetali C, Sweiss N, Amin MA, Zomorrodi RK, and Shahrara S

Subjects

Arthritis, Rheumatoid metabolism, Arthritis, Rheumatoid pathology, Cells, Cultured, Chemokine CCL2 immunology, Chemokine CCL2 metabolism, Chemokines, CC metabolism, Extracellular Signal-Regulated MAP Kinases metabolism, Fibroblasts cytology, Fibroblasts immunology, Fibroblasts metabolism, Humans, Interleukin-8 immunology, Interleukin-8 metabolism, Macrophages cytology, Macrophages metabolism, Monocytes cytology, Monocytes immunology, Monocytes metabolism, Osteoclasts cytology, Osteoclasts metabolism, Phosphorylation, Receptors, CCR metabolism, Signal Transduction immunology, Synovial Fluid cytology, Synovial Fluid immunology, Synovial Fluid metabolism, p38 Mitogen-Activated Protein Kinases metabolism, Arthritis, Rheumatoid immunology, Cell Differentiation immunology, Chemokines, CC immunology, Macrophages immunology, Osteoclasts immunology, Receptors, CCR immunology

Abstract

This study elucidates the mechanism of CCL25 and CCR9 in rheumatoid arthritis (RA). RA synovial fluid (SF) expresses elevated levels of CCL25 compared to OA SF and plasma from RA and normal. CCL25 was released into RA SF by fibroblasts (FLS) and macrophages (MΦs) stimulated with IL-1β and IL-6. CCR9 is also presented on IL-1β and IL-6 activated RA FLS and differentiated MΦs. Conversely, in RA PBMCs neither CCL25 nor CCR9 are impacted by 3-month longitudinal TNF inhibitor therapy. CCL25 amplifies RA FLS and monocyte infiltration via p38 and ERK phosphorylation. CCL25-stimulated RA FLS secrete potentiated levels of IL-8 which is disrupted by p38 and ERK inhibitors. CCL25 polarizes RA monocytes into nontraditional M1 MΦs that produce IL-8 and CCL2. Activation of p38 and ERK cascades are also responsible for the CCL25-induced M1 MΦ development. Unexpectedly, CCL25 was unable to polarize RA PBMCs into effector Th1/Th17 cells. Consistently, lymphokine like RANKL was uninvolved in CCL25-induced osteoclastogenesis; however, this manifestation was regulated by osteoclastic factors such as RANK, cathepsin K (CTSK), and TNF-α. In short, we reveal that CCL25/CCR9 manipulates RA FLS and MΦ migration and inflammatory phenotype in addition to osteoclast formation via p38 and ERK activation., (© 2021 Wiley-VCH GmbH.)

Published

2021

10. TLR7 endogenous ligands remodel glycolytic macrophages and trigger skin-to-joint crosstalk in psoriatic arthritis.

Author

Van Raemdonck K, Umar S, Palasiewicz K, Romay B, Volkov S, Arami S, Sweiss N, and Shahrara S

Subjects

Animals, Antigens, CD immunology, Antigens, Differentiation, Myelomonocytic immunology, Cytokines immunology, Humans, Inflammation immunology, Ligands, Lymphocytes immunology, Mice, Mice, Inbred DBA, MicroRNAs immunology, Myeloid Cells immunology, Osteoclasts immunology, Signal Transduction immunology, Synovial Fluid immunology, Th1 Cells immunology, Arthritis, Psoriatic immunology, Joints immunology, Macrophages immunology, Skin immunology, Toll-Like Receptor 7 immunology

Abstract

Thirty percent of psoriasis patients develop psoriatic arthritis (PsA), nevertheless the mechanism remains unknown. Endogenous GU-rich miRNAs activate endosomal TLR7 that plays a critical role in autoimmune diseases. We found that endogenous TLR7 ligands, miR-29 and miR-Let7b, were markedly increased in PsA compared to osteoarthritis (OA) synovial fluid (SF)s. We showed that intradermal (i.d.) miR-Let7b injection promoted skin inflammation, which was characterized by amplified Th1 cells, CD68 + M1 macrophages, and transcriptional upregulation of glycolytic mediators, GLUT1, C-MYC, and HIF1α. Expansion of skin Th1 cells driven by miR-Let7b was also linked to elevated M1-associated IRFs. Interestingly, i.d. miR-Let7b administration exacerbated suboptimal joint inflammation along with metabolic reconfiguration of the PsA-like preclinical model. Moreover, TLR7 agonist, R837, potentiated metabolic reprogramming and expression of IL-1β, IL-6, and IL-12 in murine macrophages, enabling myeloid-to-T-cell crosstalk. Consistently, treatment with glycolytic inhibitors, 2-DG and/or HIF1αi, reversed R837-induced metabolic remodeling and disrupted the TLR7-driven inflammatory phenotype in myeloid and lymphoid cells. Similar to miR-Let7b, R837 also differentiates progenitor cells into mature osteoclasts, primarily through RANKL induction. Taken together, this study indicates that TLR7-instigated metabolic rewiring of macrophages and their cross-regulation of T cells connects skin immunopathology to joint inflammation., (© 2020 Wiley-VCH GmbH.)

Published

2021

11. [Evaluation of a multiplex PCR assay to differentiate mycobacteria of the Mycobacterium tuberculosis complex in a reference laboratory].

Author

Arráiz R N, Romay B Z, and Faría M N

Subjects

Base Sequence, DNA, Bacterial analysis, Genome, Bacterial, Humans, Molecular Sequence Data, Mycobacterium bovis genetics, Mycobacterium bovis isolation & purification, Mycobacterium tuberculosis genetics, Mycobacterium tuberculosis isolation & purification, Oligonucleotides analysis, Tuberculosis diagnosis, Bacterial Typing Techniques, Mycobacterium bovis classification, Mycobacterium tuberculosis classification, Polymerase Chain Reaction methods, Tuberculosis microbiology

Abstract

Mycobacteria that cause tuberculosis in animals and humans belong to the Mycobacterium tuberculosis complex. Techniques for conventional diagnosis are time-consuming and do not differentiate between different strains belonging to the M. tuberculosis complex. The aim of this study was to evaluate a multiplex PCR assay applicable to mycobacteria in culture with the capacity to differentiate different strains belonging to the M. tuberculosis complex in a reference laboratory. Primers based on genomics regions of difference (RD) consisting in DNA segments that are present in M. tuberculosis, but differentially deleted in several members of M. tuberculosis complex were used in a PCR assay. The test was applied to 86 clinical isolates of mycobacteria. The pattern of amplification allowed differentiating between M. tuberculosis, M. bovis and M. bovis BCG in a single PCR reaction. This PCR multiplex assay may be used in a Reference Laboratory of Tuberculosis Diagnosis as a complementary test to differentiate mycobacteria strains belonging to the M. tuberculosis complex. This test significantly reduces the time period between culture and strain identification, and thus for could favor the adoption of better strain specific antimycobacterial regimens as well as identification of zoonotic transmission of M. bovis to humans.

Published

2007