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6. Responsiveness to osteopathic manipulative treatments in people with non-specific low back pain: A secondary analysis of the LCOSTEO trial.

Author

Rören A, Yagappa DM, Zegarra-Parodi R, Fabre L, Krief G, Daste C, Lefèvre-Colau MM, Rannou F, and Nguyen C

Subjects
Humans, Male, Female, Adult, Middle Aged, Treatment Outcome, Pain Measurement, Low Back Pain therapy, Manipulation, Osteopathic methods
Abstract

Competing Interests: Declaration of competing interest The authors have declared no conflicts of interest.

Published
2024
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7. Effect of Osteopathic Manipulative Treatment vs Sham Treatment on Activity Limitations in Patients With Nonspecific Subacute and Chronic Low Back Pain: A Randomized Clinical Trial.

Author

Nguyen C, Boutron I, Zegarra-Parodi R, Baron G, Alami S, Sanchez K, Daste C, Boisson M, Fabre L, Krief P, Krief G, Lefèvre-Colau MM, and Rannou F

Subjects
Adult, Chronic Pain epidemiology, Chronic Pain therapy, Female, Humans, Low Back Pain epidemiology, Male, Manipulation, Osteopathic statistics & numerical data, Middle Aged, Prospective Studies, Quebec, Single-Blind Method, Treatment Outcome, Low Back Pain therapy, Manipulation, Osteopathic standards, Placebos standards
Abstract

Importance: Osteopathic manipulative treatment (OMT) is frequently offered to people with nonspecific low back pain (LBP) but never compared with sham OMT for reducing LBP-specific activity limitations., Objective: To compare the efficacy of standard OMT vs sham OMT for reducing LBP-specific activity limitations at 3 months in persons with nonspecific subacute or chronic LBP., Design, Setting, and Participants: This prospective, parallel-group, single-blind, single-center, sham-controlled randomized clinical trial recruited participants with nonspecific subacute or chronic LBP from a tertiary care center in France starting February 17, 2014, with follow-up completed on October 23, 2017. Participants were randomly allocated to interventions in a 1:1 ratio. Data were analyzed from March 22, 2018, to December 5, 2018., Interventions: Six sessions (1 every 2 weeks) of standard OMT or sham OMT delivered by nonphysician, nonphysiotherapist osteopathic practitioners., Main Outcomes and Measures: The primary end point was mean reduction in LBP-specific activity limitations at 3 months as measured by the self-administered Quebec Back Pain Disability Index (score range, 0-100). Secondary outcomes were mean reduction in LBP-specific activity limitations; mean changes in pain and health-related quality of life; number and duration of sick leaves, as well as number of LBP episodes at 12 months; and consumption of analgesics and nonsteroidal anti-inflammatory drugs at 3 and 12 months. Adverse events were self-reported at 3, 6, and 12 months., Results: Overall, 200 participants were randomly allocated to standard OMT and 200 to sham OMT, with 197 analyzed in each group; the median (range) age at inclusion was 49.8 (40.7-55.8) years, 235 of 394 (59.6%) participants were women, and 359 of 393 (91.3%) were currently working. The mean (SD) duration of the current LBP episode was 7.5 (14.2) months. Overall, 164 (83.2%) patients in the standard OMT group and 159 (80.7%) patients in the sham OMT group had the primary outcome data available at 3 months. The mean (SD) Quebec Back Pain Disability Index scores for the standard OMT group were 31.5 (14.1) at baseline and 25.3 (15.3) at 3 months, and in the sham OMT group were 27.2 (14.8) at baseline and 26.1 (15.1) at 3 months. The mean reduction in LBP-specific activity limitations at 3 months was -4.7 (95% CI, -6.6 to -2.8) and -1.3 (95% CI, -3.3 to 0.6) for the standard OMT and sham OMT groups, respectively (mean difference, -3.4; 95% CI, -6.0 to -0.7; P = .01). At 12 months, the mean difference in mean reduction in LBP-specific activity limitations was -4.3 (95% CI, -7.6 to -1.0; P = .01), and at 3 and 12 months, the mean difference in mean reduction in pain was -1.0 (95% CI, -5.5 to 3.5; P = .66) and -2.0 (95% CI, -7.2 to 3.3; P = .47), respectively. There were no statistically significant differences in other secondary outcomes. Four and 8 serious adverse events were self-reported in the standard OMT and sham OMT groups, respectively, though none was considered related to OMT., Conclusions and Relevance: In this randomized clinical trial of patients with nonspecific subacute or chronic LBP, standard OMT had a small effect on LBP-specific activity limitations vs sham OMT. However, the clinical relevance of this effect is questionable., Trial Registration: ClinicalTrials.gov Identifier: NCT02034864.

Published
2021
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8. Proteomic profiling of whole-saliva reveals correlation between Burning Mouth Syndrome and the neurotrophin signaling pathway.

Author

Krief G, Haviv Y, Deutsch O, Keshet N, Almoznino G, Zacks B, Palmon A, and Aframian DJ

Subjects
Aged, Aged, 80 and over, Burning Mouth Syndrome genetics, Female, Humans, Male, Middle Aged, Nerve Growth Factors genetics, Nerve Tissue Proteins genetics, Nerve Tissue Proteins metabolism, Proteome genetics, Receptors, Nerve Growth Factor genetics, Receptors, Nerve Growth Factor metabolism, Signal Transduction, Burning Mouth Syndrome metabolism, Nerve Growth Factors metabolism, Proteome metabolism, Saliva metabolism
Abstract

Burning mouth syndrome (BMS) is characterized by a spontaneous and chronic sensation of burning in the oral mucosa, with no apparent signs. The underlying pathophysiological and neuropathic mechanisms remain unclear. Here, we attempt to elucidate some of these mechanisms using proteomic profiling and bioinformatic analyses of whole-saliva (WS) from BMS patients compared to WS from healthy individuals. Qualitative and quantitative proteomic profiling was performed using two dimensional gel electrophoresis (2-DE) and quantitative mass spectrometry (q-MS). In order to improve protein visibility, 21 high abundance proteins were depleted before proteomic profiling. Quantitative proteomic analysis revealed 100 BMS specific proteins and an additional 158 proteins up-regulated by more than threefold in those with BMS. Bioinformatic analyses of the altered protein expression profile of BMS group indicated high correlations to three cellular mechanisms including the neurotrophin signaling pathway. Based on this finding, we suggest that neurotrophin signaling pathway is involved in the pathophysiology of BMS by amplifying P75NTR activity, which in turn increases neural apoptosis thereby reducing sub-papillary nerve fiber density in the oral mucosa.

Published
2019
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9. Identification of salivary protein biomarkers for orthodontically induced inflammatory root resorption.

Author

Kaczor-Urbanowicz KE, Deutsch O, Zaks B, Krief G, Chaushu S, and Palmon A

Subjects
Biomarkers metabolism, Female, Humans, Inflammation etiology, Inflammation metabolism, Male, Proteomics, Root Resorption etiology, Root Resorption metabolism, Salivary Proteins and Peptides metabolism, Tooth Movement Techniques adverse effects
Abstract

Purpose: Orthodontically induced inflammatory root resorption (OIIRR) is one of the most prevalent and unavoidable consequence of orthodontic tooth movement. The aim of this study was to discover potential diagnostic protein biomarkers for detection of OIIRR in whole saliva (WS)., Material and Methods: Unstimulated WS was collected from 72 subjects: 48 OIIRR patients and 24 untreated, generally healthy, age and gender matched controls. Radiographic assessment of periapical x-rays of four upper incisors taken before and 9 months after bonding was done. High-abundance proteins were depleted followed by two-dimensional-gel-electrophoresis and quantitative mass spectrometry (qMS). Finally, to initially validate qMS results, Western blotting was performed., Results: qMS revealed differentially expressed proteins in the moderate-to-severe OIIRR group, which have never been found in WS before. Additionally, in the moderate-to-severe young OIIRR group, the pathogenetic mechanisms related to actin cytoskeleton regulation and Fc gamma R- mediated phagocytosis were detected, while in adults- to focal adhesion. Preliminary validation by Western blotting of fetuin-A and p21-ARC indicated expression profile trends similar to those identified by qMS., Conclusion: The significance of WS novel proteomic methodologies is clearly demonstrated for detecting new OIIRR biomarkers as well as for unveiling possible novel pathogenetic mechanisms in both young and adult patients., (© 2017 WILEY-VCH Verlag GmbH & Co. KGaA, Weinheim.)

Published
2017
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10. Identification of Sjögren's syndrome oral fluid biomarker candidates following high-abundance protein depletion.

Author

Deutsch O, Krief G, Konttinen YT, Zaks B, Wong DT, Aframian DJ, and Palmon A

Subjects
Apoptosis Regulatory Proteins metabolism, Biomarkers metabolism, Calcium-Binding Proteins metabolism, Carbonic Anhydrase I metabolism, Case-Control Studies, Female, Heat-Shock Proteins metabolism, Humans, Middle Aged, Profilins metabolism, Sensitivity and Specificity, Proteins metabolism, Proteomics methods, Saliva metabolism, Sjogren's Syndrome diagnosis, Sjogren's Syndrome metabolism
Abstract

Objective: SS is an autoimmune exocrinopathy affecting ∼1 million patients in the USA that is diagnosed mostly in middle-aged women. Oral fluids (OFs) serving as the mirror of the body were suggested as an ideal non-invasive diagnostic tool. Previously we developed depletion techniques for OF high-abundance proteins to increase visualization of low-abundance proteins. Therefore the aim of this study was to examine the effect of depletion pretreatments on the identification potential of SS OF biomarker candidates., Methods: Unstimulated OFs were collected from 18 female SS patients and 18 healthy age- and gender-matched controls. High-abundance proteins were depleted using affinity and immunodepletion methodologies followed by semi-quantitative two-dimensional gel electrophoresis and quantitative dimethylation liquid chromatography tandem mass spectrometry (LC-MS/MS). To initially validate the MS results, western blotting was performed., Results: The use of depletion strategy before proteomics analysis increased identification ability by 3-fold. Overall, 79 biomarker candidates were identified. Proteins with the most pronounced fold changes were related to SS serum or tissue factors. In addition, bioinformatics analysis of proteins with a >3-fold increase in SS patients showed calcium-binding proteins, defence-response proteins, proteins involved in apoptotic regulation, stress-response proteins and cell motion-related proteins. Preliminary validation by western blotting of profilin and CA-I indicated similar expression profile trends to those identified by quantitative MS., Conclusion: The significance of OF novel depletion methodologies is clearly demonstrated for increased visibility of biomarker candidates as well as for unveiling possible mechanisms involved in this syndrome. This represents a major contribution to our ability to use OF as a future diagnostic fluid., (© The Author 2014. Published by Oxford University Press on behalf of the British Society for Rheumatology. All rights reserved. For Permissions, please email: journals.permissions@oup.com.)

Published
2015
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11. Comparison of diverse affinity based high-abundance protein depletion strategies for improved bio-marker discovery in oral fluids.

Author

Krief G, Deutsch O, Zaks B, Wong DT, Aframian DJ, and Palmon A

Subjects
Adult, Body Fluids, Combinatorial Chemistry Techniques, Electrophoresis, Gel, Two-Dimensional, Humans, Male, Biomarkers analysis, Proteins isolation & purification, Proteomics methods, Saliva chemistry
Abstract

Oral fluids (OF) have been suggested as a source of biomarkers for oral and systemic health, but as with other bio-fluids, the presence of high-abundance proteins interferes with the detection of lower-abundance biomarkers. Here, we compared the performance of four depletion treatments: triple depletion (TD) of amylases, albumins and immunoglobulin G; multiple depletion (MD) of amylases and a panel of 20 proteins, a combination of the two (EMD) and combinatorial peptide ligand library based depletion termed CPLL. TD, MD, EMD and CPLL removed 76%, 83%, 85% and 94% of total proteins, respectively, coupled with increased low abundance protein detection and narrowed dynamic range. 2-DE revealed that all depletion pretreatments successfully clarified areas hampered by high-abundance proteins; however, EMD and CPLL exposed the highest number of proteins. Quantitative MS of EMD samples relative to none treated samples indicated that most of downregulated proteins (>90%) were EMD target proteins. In conclusion, a multiple step EMD and CPLL depletion approaches bring about the highest number of protein detection ability and the best hampered-area clearance. As CPLL requires at least 10 fold more protein starting material, we suggest EMD pretreatment as a new detection tool in instances of low protein starting material., (Copyright © 2012 Elsevier B.V. All rights reserved.)

Published
2012
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12. High-efficiency immunomagnetic isolation of solid tissue-originated integrin-expressing adult stem cells.

Author

Palmon A, David R, Neumann Y, Stiubea-Cohen R, Krief G, and Aframian DJ

Subjects
Affinity Labels chemistry, Animals, Antibodies, Monoclonal chemistry, Cell Membrane chemistry, Cell Survival, Flow Cytometry, Head and Neck Neoplasms chemistry, Humans, Male, Rats, Rats, Sprague-Dawley, Salivary Glands chemistry, Salivary Glands pathology, Sensitivity and Specificity, Adult Stem Cells chemistry, Immunomagnetic Separation methods, Integrin alpha6beta1 chemistry
Abstract

Isolation of highly pure specific cell types is crucial for successful adult stem cell-based therapy. As the number of such cells in adult tissue is low, an extremely efficient method is needed for their isolation. Here, we describe cell-separation methodologies based on magnetic-affinity cell sorting (MACS) MicroBeads with monoclonal antibodies against specific membrane proteins conjugated to superparamagnetic particles. Cells labeled with MACS MicroBeads are retained in a magnetic field within a MACS column placed in a MACS separator, allowing fast and efficient separation. Both positively labeled and non-labeled fractions can be used directly for downstream applications as the separated cell fractions remain viable with no functional impairment. As immunomagnetic separation depends on the interaction between a cell's membrane and the magnetically labeled antibody, separation of specific cells originating from solid tissues is more complex and demands a cell-dissociating pretreatment. In this paper, we detail the use of immunomagnetic separation for the purpose of regenerating damaged salivary gland (SG) function in animal and human models of irradiated head and neck cancer. Each year 500,000 new cases of head and neck cancer occur worldwide. Most of these patients lose SG function following irradiation therapy. SGs contain integrin α6β1-expressing epithelial stem cells. We hypothesized that these cells can be isolated, multiplied in culture and auto-implanted into the irradiated SGs to regenerate damaged SG function., (Copyright © 2011 Elsevier Inc. All rights reserved.)

Published
2012
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13. Effect of irradiation on cell transcriptome and proteome of rat submandibular salivary glands.

Author

Stiubea-Cohen R, David R, Neumann Y, Krief G, Deutsch O, Zacks B, Aframian DJ, and Palmon A

Subjects
Animals, Cluster Analysis, Female, Gene Expression Profiling, Gene Expression Regulation radiation effects, Rats, Rats, Sprague-Dawley, Saliva metabolism, Time Factors, Proteome radiation effects, Submandibular Gland metabolism, Submandibular Gland radiation effects, Transcriptome radiation effects
Abstract

Salivary glands (SGs) are irreversibly damaged by irradiation (IR) treatment in head and neck cancer patients. Here, we used an animal irradiation model to investigate and define the molecular mechanisms affecting SGs following IR, focusing on saliva proteome and global transcription profile of submandibular salivary gland (SSG) tissue.We show that saliva secretion was gradually reduced to 50% of its initial level 12 weeks post-IR. Saliva protein composition was further examined by proteomic analysis following mass spectrometry (MS) analysis that revealed proteins with reduced expression originating from SSGs and proteins with increased expression derived from the serum, both indicating salivary tissue damage. To examine alterations in mRNA expression levels microarray analysis was performed. We found significant alterations in 95 genes, including cell-cycle arrest genes, SG functional genes and a DNA repair gene.Tissue damage was seen by confocal immunofluorescence of α-amylase and c-Kit that showed an increase and decrease, respectively, in protein expression. This was coherent with real-time PCR results.This data indicates that IR damages the SSG cells' ability to produce and secrete saliva and proteins, and maintain the physiological barrier between serum and saliva. The damage does not heal due to cell-cycle arrest, which prevents tissue regeneration. Taken together, our results reveal a new insight into IR pathobiology.

Published
2012
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14. An approach to remove alpha amylase for proteomic analysis of low abundance biomarkers in human saliva.

Author

Deutsch O, Fleissig Y, Zaks B, Krief G, Aframian DJ, and Palmon A

Subjects
Adsorption, Biomarkers analysis, Electrophoresis, Polyacrylamide Gel, Humans, Starch chemistry, Proteome analysis, Proteomics methods, Saliva chemistry, alpha-Amylases isolation & purification
Abstract

Proteomic characterization of human whole saliva for the identification of disease-specific biomarkers is guaranteed to be an easy-to-use and powerful diagnostic tool for defining the onset, progression and prognosis of human systemic diseases and, in particular, oral diseases. The high abundance of proteins, mainly alpha amylase, hampers the detection of low abundant proteins appearing in the disease state and therefore should be removed. In the present study a 2-DE was used to analyze human whole saliva following the removal of alpha amylase by affinity adsorption to potato starch. After alpha amylase removal whole saliva was analyzed by SDS-PAGE showing at least sixfold removal efficiency and by an alpha amylase activity assay showing 97% reduced activity. MS identification of the captured alpha amylase after elution demonstrated specific removal; 2-DE analysis showed the selective removal of alpha amylase and consequently increased gel resolution. MS identification of protein spots in the 60 kDa area revealed 15 proteins, which were masked before alpha amylase removal. In conclusion, treatment of human whole saliva with an alpha amylase removal device increases gel resolution and enables a higher protein sample for analysis.

Published
2008
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17. [Update on clasps].

Author

Doukhan JY, Kleinfinger S, Krief G, and Levavasseur F

Subjects
Denture Design, Humans, Denture Retention, Denture, Partial, Removable
Published
1988

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