Restoring Specific Lactobacilli Levels Decreases Inflammation and Muscle Atrophy Markers in an Acute Leukemia Mouse Model

The gut microbiota has recently been proposed as a novel component in the regulation of host homeostasis and immunity. We have assessed for the first time the role of the gut microbiota in a mouse model of leukemia (transplantation of BaF3 cells containing ectopic expression of Bcr-Abl), characterized at the final stage by a loss of fat mass, muscle atrophy, anorexia and inflammation. The gut microbial 16S rDNA analysis, using PCR-Denaturating Gradient Gel Electrophoresis and quantitative PCR, reveals a dysbiosis and a selective modulation of Lactobacillus spp. (decrease of L. reuteri and L. johnsonii/gasseri in favor of L. murinus/animalis) in the BaF3 mice compared to the controls. The restoration of Lactobacillus species by oral supplementation with L. reuteri 100-23 and L. gasseri 311476 reduced the expression of atrophy markers (Atrogin-1, MuRF1, LC3, Cathepsin L) in the gastrocnemius and in the tibialis, a phenomenon correlated with a decrease of inflammatory cytokines (interleukin-6, monocyte chemoattractant protein-1, interleukin-4, granulocyte colony-stimulating factor, quantified by multiplex immuno-assay). These positive effects are strain- and/or species-specific since L. acidophilus NCFM supplementation does not impact on muscle atrophy markers and systemic inflammation. Altogether, these results suggest that the gut microbiota could constitute a novel therapeutic target in the management of leukemia-associated inflammation and related disorders in the muscle

HIV-1 assembly in macrophages

The molecular mechanisms involved in the assembly of newly synthesized Human Immunodeficiency Virus (HIV) particles are poorly understood. Most of the work on HIV-1 assembly has been performed in T cells in which viral particle budding and assembly take place at the plasma membrane. In contrast, few studies have been performed on macrophages, the other major target of HIV-1. Infected macrophages represent a viral reservoir and probably play a key role in HIV-1 physiopathology. Indeed macrophages retain infectious particles for long periods of time, keeping them protected from anti-viral immune response or drug treatments. Here, we present an overview of what is known about HIV-1 assembly in macrophages as compared to T lymphocytes or cell lines

Identification of heparin-binding EGF-like growth factor (HB-EGF) as a biomarker for lysophosphatidic acid receptor type 1 (LPA1) activation in human breast and prostate cancers

Lysophosphatidic acid (LPA) is a natural bioactive lipid with growth factor-like functions due to activation of a series of six G protein-coupled receptors (LPA₁₋₆). LPA receptor type 1 (LPA₁) signaling influences the pathophysiology of many diseases including cancer, obesity, rheumatoid arthritis, as well as lung, liver and kidney fibrosis. Therefore, LPA₁ is an attractive therapeutic target. However, most mammalian cells co-express multiple LPA receptors whose co-activation impairs the validation of target inhibition in patients because of missing LPA receptor-specific biomarkers. LPA₁ is known to induce IL-6 and IL-8 secretion, as also do LPA₂ and LPA₃. In this work, we first determined the LPA induced early-gene expression profile in three unrelated human cancer cell lines expressing different patterns of LPA receptors (PC3: LPA₁,₂,₆; MDA-MB-231: LPA1,2; MCF-7: LPA₂,₆). Among the set of genes upregulated by LPA only in LPA₁-expressing cells, we validated by QPCR and ELISA that upregulation of heparin-binding EGF-like growth factor (HB-EGF) was inhibited by LPA₁-₃ antagonists (Ki16425, Debio0719). Upregulation and downregulation of HB-EGF mRNA was confirmed in vitro in human MDA-B02 breast cancer cells stably overexpressing LPA₁ (MDA-B02/LPA₁) and downregulated for LPA₁ (MDA-B02/shLPA1), respectively. At a clinical level, we quantified the expression of LPA₁ and HB-EGF by QPCR in primary tumors of a cohort of 234 breast cancer patients and found a significantly higher expression of HB-EGF in breast tumors expressing high levels of LPA₁. We also generated human xenograph prostate tumors in mice injected with PC3 cells and found that a five-day treatment with Ki16425 significantly decreased both HB-EGF mRNA expression at the primary tumor site and circulating human HB-EGF concentrations in serum. All together our results demonstrate that HB-EGF is a new and relevant biomarker with potentially high value in quantifying LPA₁ activation state in patients receiving anti-LPA₁ therapies

Autotaxin in cancer cell dissemination to the bone : involvement of blood platelets, alphaV/Beta3 integrin and Syndecan-4

L'autotaxine (ATX) est une glycoprotéine sécrétée qui grâce à son activité lysophospholipase D est à l'origine d'un lipide biologiquement actif, l'acide lysophosphatidique (LPA), dans la circulation sanguine. L'expression de l'ATX par les cellules tumorales contrôle la dissémination métastatique spontanée des cellules de cancer du sein et la formation des métastases osseuses. Au cours de cette thèse, nous avons observé que le ciblage thérapeutique précoce de l'ATX dans un modèle animal préclinique bloque de façon remarquable la dissémination métastatique des cellules de cancer du sein. Cependant les mécanismes moléculaires à l'origine de l'action du LPA sur les cellules tumorales sont mal caractérisés. Nous avons ici montré, via des expériences in vitro et in vivo, que l'ATX circulante d'origine non tumorale libérée par les plaquettes sanguines sous l'action des cellules tumorales, contrôle les évènements précoces de la dissémination métastatique. Cependant, le LPA est un lipide extrêmement sensible à l'action des phosphatases, présentes en grande quantité dans les milieux extracellulaires : l'activité du LPA serait dépendante de sa production locale, au voisinage de ses récepteurs présents à la surface des cellules. Ces travaux ont ainsi mis en évidence que le pouvoir pro-métastatique de l'ATX dépend à la fois de son interaction avec l'intégrine Alpha V/Beta3exprimée par les cellules tumorales, mais également d'un protéoglycane, Syndecan-4 présent en surface cellulaire. En conclusion, le ciblage de l’ATX via son activité ou via ses interactions présente un haut potentiel thérapeutique chez des patientes atteintes d'un cancer du sein à fort risque métastatiqueBone metastases are a frequent complication of cancer, occurring in up to 70 percent of patients with advanced breast or prostate cancer. Despite the improvement of current therapies, the survival of bone metastasis patients is only 24 months. This study aims to find new mechanisms involved in bone metastasis formation. Autotaxin (ATX/NPP2) is a secreted glycoprotein that generates lysophosphatidic acid (LPA) through its lysophospholipase D activity. Our lab previously demonstrated that ATX is overexpressed in multiple types of cancers and together with LPA generated during platelet activation promotes skeletal metastasis of breast cancer. However, the pathophysiological sequelae of regulated interactions between circulating LPA, ATX and platelets remain undefined in cancer. In this work we show that ATX is stored in a- granules of resting human platelets and released upon tumor cell-induced platelet aggregation, leading to the production of LPA. Our in vitro and in vivo experiments using human breast cancers cells that do not express ATX demonstrate that non-tumoral ATX controls the early stage of bone colonization by tumor cells. However, LPA is extremely sensitive to phosphatases, which are highly expressed in extracellular environment and at cell membranes. The molecular mechanisms involved in the local production of LPA at the bone metastatic site are still not well characterized. The present results establish that binding of ATX to alphaV/Beta3 integrin and/or the proteoglycan syndecan-4 allow LPA delivery to its receptors present at the surface of tumor cells. These results may have important implications in the development of new therapies for patients with bone metastase

Rôle de l'autotaxine dans la dissémination métastatique à l'os : implication des plaquettes sanguines, de l'intégrine Alpha V/Beta3 et du protéoglycane syndecan-4

Bone metastases are a frequent complication of cancer, occurring in up to 70 percent of patients with advanced breast or prostate cancer. Despite the improvement of current therapies, the survival of bone metastasis patients is only 24 months. This study aims to find new mechanisms involved in bone metastasis formation. Autotaxin (ATX/NPP2) is a secreted glycoprotein that generates lysophosphatidic acid (LPA) through its lysophospholipase D activity. Our lab previously demonstrated that ATX is overexpressed in multiple types of cancers and together with LPA generated during platelet activation promotes skeletal metastasis of breast cancer. However, the pathophysiological sequelae of regulated interactions between circulating LPA, ATX and platelets remain undefined in cancer. In this work we show that ATX is stored in a- granules of resting human platelets and released upon tumor cell-induced platelet aggregation, leading to the production of LPA. Our in vitro and in vivo experiments using human breast cancers cells that do not express ATX demonstrate that non-tumoral ATX controls the early stage of bone colonization by tumor cells. However, LPA is extremely sensitive to phosphatases, which are highly expressed in extracellular environment and at cell membranes. The molecular mechanisms involved in the local production of LPA at the bone metastatic site are still not well characterized. The present results establish that binding of ATX to alphaV/Beta3 integrin and/or the proteoglycan syndecan-4 allow LPA delivery to its receptors present at the surface of tumor cells. These results may have important implications in the development of new therapies for patients with bone metastasesL'autotaxine (ATX) est une glycoprotéine sécrétée qui grâce à son activité lysophospholipase D est à l'origine d'un lipide biologiquement actif, l'acide lysophosphatidique (LPA), dans la circulation sanguine. L'expression de l'ATX par les cellules tumorales contrôle la dissémination métastatique spontanée des cellules de cancer du sein et la formation des métastases osseuses. Au cours de cette thèse, nous avons observé que le ciblage thérapeutique précoce de l'ATX dans un modèle animal préclinique bloque de façon remarquable la dissémination métastatique des cellules de cancer du sein. Cependant les mécanismes moléculaires à l'origine de l'action du LPA sur les cellules tumorales sont mal caractérisés. Nous avons ici montré, via des expériences in vitro et in vivo, que l'ATX circulante d'origine non tumorale libérée par les plaquettes sanguines sous l'action des cellules tumorales, contrôle les évènements précoces de la dissémination métastatique. Cependant, le LPA est un lipide extrêmement sensible à l'action des phosphatases, présentes en grande quantité dans les milieux extracellulaires : l'activité du LPA serait dépendante de sa production locale, au voisinage de ses récepteurs présents à la surface des cellules. Ces travaux ont ainsi mis en évidence que le pouvoir pro-métastatique de l'ATX dépend à la fois de son interaction avec l'intégrine Alpha V/Beta3exprimée par les cellules tumorales, mais également d'un protéoglycane, Syndecan-4 présent en surface cellulaire. En conclusion, le ciblage de l’ATX via son activité ou via ses interactions présente un haut potentiel thérapeutique chez des patientes atteintes d'un cancer du sein à fort risque métastatiqu

Errors in the knee joint forces and moments during gait depending on the foot and knee prosthetic components from stabilisation during gain stance

XV World Congress of the International Society for Prosthetics and Orthotics (ISPO), LYON, FRANCE, 22-/06/2015 - 25/06/2015Previously studies showed that inverse dynamics based on motion analysis and force - plate is inaccurate compared to direct measurements for individuals with transfemoral amputation (TFA). Indeed, direct measurements can appropriately take into account the absorption at the prosthetic foot and the resistance at the prosthetic knee. However, these studies involved only a passive prosthetic kne

Hip power analysis in individuals with transfemoral amputation: a different strategy from stabilisation during gait stance

XXV Congress of the International Society of Biomechanics, GLASGOW, ROYAUME-UNI, 12-/07/2015 - 16/07/2015Joint moments and joint powers during gait are widely used to determine the effects of rehabilitation programs as well as prosthetic fitting. Following the definition of power (dot product of joint moment and joint angular velocity) it has been previously proposed to analyse the 3D angle between both vectors, ?Mw. Basically, joint power is maximised when both vectors are parallel and cancelled when both vectors are orthogonal. In other words, ?Mw < 60° reveals a propulsion configuration (more than 50% of the moment contribute to positive power) while ?Mw > 120° reveals a resistance configuration (more than 50% of the moment contribute to negative power). A stabilisation configuration (less than 50% of the moment contribute to power) corresponds to 60° < ?Mw < 120°. Previous studies demonstrated that hip joints of able - bodied adults (AB) are mainly in a stabilisation configuration (?Mw about 90°) during the stance phase of gait. Individuals with transfemoral amputation (TFA) need to maximise joint power at the hip while controlling the prosthetic knee during stance. Therefore, we tested the hypothesis that TFAs should adopt a strategy that is different from a continuous stabilisation. The objective of this study was to compute joint power and ?Mw for TFA and to compare them with A

Importance of quorum sensing crosstalk in the brown alga Saccharina latissima epimicrobiome

Summary: Brown macroalgae are colonized by diverse microorganisms influencing the physiology of their host. However, cell-cell interactions within the surface microbiome (epimicrobiome) are largely unexplored, despite the significance of specific chemical mediators in maintaining host-microbiome homeostasis. In this study, by combining liquid chromatography coupled to mass spectrometry (LC-MS) analysis and bioassays, we demonstrated that the widely diverse fungal epimicrobiota of the brown alga Saccharina latissima can affect quorum sensing (QS), a type of cell-cell interaction, as well as bacterial biofilm formation. We also showed the ability of the bacterial epimicrobiota to form and inhibit biofilm growth, as well as to activate or inhibit QS pathways. Overall, we demonstrate that QS and anti-QS compounds produced by the epimicrobiota are key metabolites in these brown algal epimicrobiota communities and highlight the importance of exploring this epimicrobiome for the discovery of new bioactive compounds, including potentially anti-QS molecules with antifouling properties

Pharmacological blockade of LPA₁<i>in vivo</i> inhibits HB-EGF secretion by human PC3 xenographs.

<p>PC3 tumor cells were injected subcutaneously in the right flank of male BALB/C nude mice. At day 35, post-tumor cell injection animals were randomized into two groups and treated with Ki16425 (25 mg/kg) or the vehicle for 5 d. (A) Representative photographs of primary tumors at day 40 (upper panels). Box plot represent tumor volumes (in mm³) (lower panels). Bar represents 10 mm. (B) <i>LPAR1</i>, <i>LPAR2</i> and <i>LPAR3</i> expressions were measured by real-time quantitative PCR and normalized to housekeeping <i>L32</i> gene values (Veh: Vehicle; Ki: Ki16425) (C) Box plot represents expression of HB-EGF mRNA expression detected by real-time quantitative PCR from total RNAs isolated from tumors of animals treated with vehicle or Ki16425. Values were normalized to housekeeping L32 gene. ¶: <i>p</i><0.05, using unpaired Student t-Test. (D) Box plot represents HB-EGF concentration detected by ELISA in the serum of animals treated with Ki16425 or vehicle. ¶: <i>p</i><0.05, using unpaired Student t-Test.</p