Activité anti-tumorale d’une matrikine dérivée des domaines NC1 du collagène IV de membrane basale / Anti-tumor activity of a matrikine derived from NC1 domains of basement membrene collagen IV

Senechal, Karine

09 December 2011

Le mélanome est le cancer cutané le plus invasif. Au cours de l’invasion tumorale et de la dissémination métastatique, les cellules tumorales sont capables de dégrader la matrice extracellulaire par la sécrétion de protéases telles que les MMPs. Lors de cette protéolyse matricielle, différents fragments de la matrice extracellulaire exerçant des activités anti-tumorale et/ou anti-angiogénique, nommés matrikines, sont libérés et modulent la croissance tumorale. De nombreuses matrikines dérivées des collagènes de membrane basale sont capables de limiter la progression tumorale. Nous avons étudié les propriétés anti-tumorales du domaine NC1 α4(IV), nommé tétrastatine, à la fois in vitro et in vivo dans un modèle de mélanome humain. La tétrastatine induit une inhibition de la prolifération et de l’invasion des cellules de mélanome in vitro. L’inhibition de prolifération est corrélée à un retard en phase G1/S du cycle cellulaire en présence de tétrastatine. L’inhibtion de l’invasion peut notamment s’expliquer par une inhibition de l’activation de la MMP-14 et une modification de sa répartition cellulaire, avec perte du phénotype migratoire en présence de tétrastatine. In vivo, la surexpression de la tétrastatine induit une forte inhibition de la croissance tumorale, dans un modèle de xénogreffe de mélanome humain chez la souris nude. Nous avons également pu identifier l’intégrine αvβ3 comme un récepteur potentiel de la tétrastatine. Enfin, l’étude des capacités anti-prolifératives et anti-invasives des cellules UACC 903 en présence de différents peptides permet aujourd’hui de mieux préciser la séquence responsable de l’activité anti-tumorale de ce domaine. En conclusion, la tétrastatine est une nouvelle matrikine à fort potentiel anti-tumoral capable de limiter la progression du mélanome. / Melanoma is the most invasive cutaneous cancer. During tumor invasion and metastatic dissemination, tumor cells degrade the extracellular matrix by secretion of proteases such as MMPs. During matrix proteolysis, fragments of the extracellular matrix with anti-tumor and/or anti-angiogenic activities, called matrikines, are released and modulate tumor growth. Many matrikines derived from basement membrane collagens are able to inhibit tumor progression. We studied the anti-tumor properties of the domain NC1 α4 (IV), named tetrastatin, both in vitro and in vivo in a human melanoma model. Tetrastatin induces inhibition of proliferation and invasion of melanoma cells in vitro. This inhibition of proliferation is correlated to a cell cycle delay in G1/S phase when cells are incubated with tetrastatin. The inhibition of invasion could be due, at least partly, to the inhibition of MMP-14 active form and modification of its cellular distribution, with a loss of the migratory phenotype in the presence of tetrastatin. In vivo, tetrastatin overexpression induces a strong inhibition of tumor growth, in a human melanoma xenograft model in nude mice. We also identified integrin αvβ3 as a potential receptor of tetrastatin. Finally, the study of the anti-proliferative and anti-invasive properties of the UACC 903 cells in the presence of different peptides allows us to better identify the sequence responsible of the anti-tumor activity. In conclusion, tetrastatin is a new potent anti-tumor matrikine capable of limiting melanoma progression.

Collagène IV

Anti-tumoral

Membrane basale

Domaine NC1

Collagen type iv

Antibodies, neoplasm

Basement membrane

Estudo da relaÃÃo do Infiltrado InflamatÃrio Mononuclear e ExpressÃo de Ki-67, ColÃgeno IV e Laminina em Cistos Radiculares / Study Of The Relationship of Mononuclear Inflammatory Infiltrade and Ki-67, Laminin And Colagem Type IV expression in radicular Cysts

Renata Veras Carvalho MourÃo

19 February 2013

CoordenaÃÃo de AperfeiÃoamento de Pessoal de NÃvel Superior / Os cistos dos ossos maxilares sÃo classificados como odontogÃnicos e nÃo odontogÃnicos. Dentre os odontogÃnicos inflamatÃrios, destaca-se o cisto radicular, e entre os de desenvolvimento, o dentÃgero. Estes cistos e suas variantes apresentam etiopatogÃnese e comportamento biolÃgico diferentes, mas sÃo igualmente lÃticos. A atividade proliferativa do epitÃlio de revestimento, dos componentes da membrana basal e da matriz extracelular, possivelmente, interferem nos mecanismos de crescimento, constituindo alvos de pesquisas. Este trabalho teve por objetivo avaliar a relaÃÃo do infiltrado inflamatÃrio mononuclear com a expressÃo de marcadores de proliferaÃÃo (Ki 67) e das proteÃnas da membrana basal e matriz extracelular nos cistos radiculares. Trata-se de um estudo retrospectivo e observacional tendo sido realizado um levantamento dos casos catalogados no ServiÃo de Biopsia do Departamento de Patologia e Medicina Legal (FAMED) e no LaboratÃrio de Patologia Bucal (FFOE) (UFC). ApÃs a revisÃo histolÃgica, os grupos foram divididos em cisto radicular intensamente inflamado (CRII) (n=17), cisto radicular levemente inflamado(CRLI)(n=.9) e cisto dentÃgero (CD) (n= 9). A presenÃa e intensidade do infiltrado inflamatÃrio histiolinfoplasmocitÃrio e preservaÃÃo do epitÃlio de revestimento foram os parÃmetros utilizados para seleÃÃo dos casos. Os espÃcimes foram submetidos à reaÃÃo de imuno-histoquÃmica por estreptoavidina biotina, utilizando-se os anticorpos Ki 67 (DakoÂ, 1:50), anti-colÃgeno IV (DBSÂ, 1:40) e anti-laminina (DBSÂ, 1:20). A expressÃo de Ki 67 foi mais intensa no grupo CRLI, quando comparada ao grupo CRII e CD. A expressÃo de colÃgeno tipo IV na membrana basal foi significante no grupo CRLI, quando comparada com o grupo CRII e CD. Jà a imunomarcaÃÃo de matriz extracelular variou de ausente a fraca nos grupos CRII e CRLI, enquanto no CD se exibiu de forma fraca a moderada, sendo esta diferenÃa significativa. A expressÃo de laminina em membrana basal nos grupos CRII e CD foi negativa e no grupo dos CRLI foi fraca e pontual. Concluiu-se que a presenÃa e a intensidade do conteÃdo inflamatÃrio na parede dos cistos radiculares parecem modificar a expressÃo dos fatores de proliferaÃÃo no epitÃlio de revestimento, e colÃgeno tipo IV e laminina na membrana basal, mas nÃo interferem no comportamento do colÃgeno IV da matriz extracelular nos cistos radiculares. A expressÃo de componentes da membrana basal (laminina e colÃgeno tipo IV) à maior nos cistos radiculares com leve infiltrado inflamatÃrio. / Jawbone cysts are classified as odontogenic and non-odontogenic cysts. The radicular cyst is the most common odontogenic cyst of inflammatory origin, whereas the detigerous cyst is the most common type of developmental odontogenic cyst. These cysts and their variations have different etiopathogenesis and biological behavior, but are equally lytic. The proliferation activity of the epithelial lining and the components of the basement membrane and extracellular matrix constitute targets of research. The aim of this study was to evaluate the relation between mononuclear inflammatory infiltrate and the expression of proliferative immunomarkers (Ki 67), and proteins of basement membrane and extracellular matrix in radicular cysts. In this retrospective observational study, all cases of jawbone cysts that had been recorded in the files of the Department of Pathology and Legal Medicine (FAMED), and of the Laboratory of Oral Pathology (FFOE) of the Federal University of Cearà (UFC) and reviewed. After histological revision, the groups were divided into heavily inflamed radicular cysts (HIRC) (n=17), slightly inflamed radicular cysts (SIRC) (n=9) and dentigerous cysts (DC) (n=9). The presence and intensity of the lymphoplasmacytic inflammatory infiltrate and the preservation of the epithelial lining were the parameters used to select the cases. Immunohistochemical analyses were performed using the standard streptavidin-biotin-peroxidase method. The primary antibodies used in this study included Ki 67 (DakoÂ, 1:50), Anti-Collagen Type IV (DBSÂ, 1:40) and Anti- Laminin (DBSÂ, 1:20).The immunoexpression of Ki-67 was more intense in the SIRC group compared to the HIRC group and DC. Likewise, the immunoexpression of Anti-Collagem Type IV in the basement membrane of the SIRC group presented a statistically significant difference compared to the HIRC group and DC . The expression of laminin in the basement membrane and in group HIRC and DC was negative and the group of SIRC was weak and punctual. It was concluded that presence and severity of inflammatory content wall of radicular cysts appear to modify the expression of proliferation factors in the coating epithelium and collagen type IV and laminin in the basement membrane but not modific with the behavior of extracellular matrix in radicular cyst. The expression of basement membrane components (laminin and collage type IV) is higher in radicular cyst with mild inflammatory infiltrade.

Immunohistochemistry

Ki-67 antigen

Laminin

Collagen type IV

Radicular Cyst

ANATOMIA PATOLOGICA E PATOLOGIA CLINICA

The sandwich theory:a bioactivity based explanation for posterior capsule opacification after cataract surgery with intraocular lens implantation

Linnola, R. (Reijo)

04 May 2001

Abstract This study was undertaken to identify mechanisms of adhesion of intraocular lenses (IOLs) to the capsular bag after cataract surgery and IOL implantation. It was also done to challenge the sandwich theory presented for posterior capsular opacification (PCO): If the IOL is made of a bioactive material it would allow a single lens epithelial cell layer to bond both to the IOL and the posterior capsule at the same time. This would produce a sandwich pattern including the IOL, the cell monolayer and the posterior capsule. The sealed sandwich structure would prevent further epithelial ingrowth. The degree of bioactivity of the IOL could explain the basic difference in the incidence of PCO and capsulotomy rates with different IOL materials. The sandwich theory was put forward on the basis of a search for a keratoprosthesis material, which would allow maximal adhesion of the prosthesis to corneal tissue. Titanium and glass-ceramic coated titanium were found to develop better adhesion than poly (methyl methacrylate) (PMMA). The adhesion of PMMA to the corneal stromal tissue was loose, and down growth of corneal epithelial cells was seen around the prosthesis. The differences between various IOL materials were first tested with rabbit corneal tissue cultures. There was better adhesion of corneal tissue to soft, hydrophobic acrylate than to PMMA, heparin surface modified (HSM)-PMMA, silicone or hydrogel IOLs. To assess differences in protein adhesion to IOL surfaces, different IOLs were incubated for 24 hours with radioactive iodine labeled fibronectin. Soft hydrophobic acrylate (AcrySof®) showed the highest binding of fibronectin, and the differences relative to all the other materials were significant (p < 0.01-0.001), except to PMMA (p = 0.31). The sandwich theory and the results with rabbit corneal tissue cultures and the protein adhesion study in vitro were evaluated against the results found in pseudophakic autopsy eyes. Altogether, 70 autopsy eyes were analyzed. From 38 autopsy eyes containing PMMA, silicone, soft hydrophobic acrylate or hydrogel IOLs histological sections were prepared from the capsular bag and immunohistochemical analyses were performed for fibronectin, vitronectin, laminin and collagen type IV. A total of 152 specimens were analyzed. From 32 autopsy eyes containing IOLs made of PMMA, silicone, acrylate or hydrogel, IOLs were explanted from the capsular bag and immunohistochemical analysis was done on both sides of the IOLs for fibronectin, vitronectin, laminin or collagen type IV. Soft hydrophobic acrylate IOLs had significantly more adhesion of fibronectin to their surfaces than PMMA or silicone IOLs. Also, more vitronectin was attached to acrylate IOLs than to the other IOL materials. Silicone IOLs had more collagen type IV adhesion in comparison to the other IOL materials studied. In histologic sections a sandwich-like structure (anterior or posterior capsule-fibronectin-one cell layer-fibronectin-IOL surface) was seen significantly more often in eyes with acrylate IOLs than in PMMA, silicone or hydrogel IOL eyes. These studies support the sandwich theory for posterior capsule opacification after cataract surgery with IOLs. The results suggest that fibronectin may be the major extracellular protein responsible for the attachment of acrylate IOLs to the capsular bag. This may represent a true bioactive bond between the IOL and the lens epithelial cells, and between the IOL and the capsular bag. This may explain the reason for clinical observations of less posterior capsular opacification and lower capsulotomy rates with the soft hydrophobic acrylate material of AcrySof® IOLs compared to the other IOL materials studied.

cataract surgery

collagen type IV

fibronectin

intraocular lenses

laminin

posterior capsule opacification

vitronectin

Effects of Chemical and Radiation Sterilisation on the Biological and Biomechanical Properties of Decellularised Porcine Peripheral Nerves

Holland, J.D.R., Webster, G., Rooney, P., Wilshaw, Stacy-Paul, Jennings, L.M., Berry, H.E.

29 June 2021

yes / There is a clinical need for novel graft materials for the repair of peripheral nerve defects. A decellularisation process has been developed for porcine peripheral nerves, yielding a material with potentially significant advantages over other devices currently being used clinically (such as autografts and nerve guidance conduits). Grafts derived from xenogeneic tissues should undergo sterilisation prior to clinical use. It has been reported that sterilisation methods may adversely affect the properties of decellularised tissues, and therefore potentially negatively impact on the ability to promote tissue regeneration. In this study, decellularised nerves were produced and sterilised by treatment with 0.1% (v/v) PAA, gamma radiation (25-28 kGy) or E Beam (33-37 kGy). The effect of sterilisation on the decellularised nerves was determined by cytotoxicity testing, histological staining, hydroxyproline assays, uniaxial tensile testing, antibody labelling for collagen type IV, laminin and fibronectin in the basal lamina, and differential scanning calorimetry. This study concluded that decellularised nerves retained biocompatibility following sterilisation. However, sterilisation affected the mechanical properties (PAA, gamma radiation), endoneurial structure and basement membrane composition (PAA) of decellularised nerves. No such alterations were observed following E Beam treatment, suggesting that this method may be preferable for the sterilisation of decellularised porcine peripheral nerves.

Peripheral nerves

Porcine peripheral nerves

Decellularisation

Sterilisation

Collagen type IV

Biomechanical properties

Radiation sterilisation

E Beam sterilisation

Migration on extracellular matrix surface and infiltration into matrix - two distinguishable activities of human T cells

Ivanoff, Jyrki

January 2003

<p>Migration of T-lymphocytes on a surface coated with extracellular matrix (ECM) components (two-dimensional (2-D) migration) and migration (infiltration) into a matrix (Three-dimesional (3-D) migration) are complex events and the underlying mechanisms are not yet fully understood. Here 2-D and 3-D migration were studied by use of seven leukemic T-cell lines representing discrete differentiation stages, a non-leukemic T-cell clone, and normal peripheral blood T cells. peripheral blood lymphocytes and the T-cell clone produced nanogram quantities of various chemokines, as compared to a production of ≤ 0.05 ng/ml by the T leukemia cell lines. In a Boyden chamber system, the leukemic T-cell lines showed haptotactic migration on fibronectin. The migration was augmented bu exposure to chemokines, including RANTES, MIP-1α, MIP-1β, and IL-8. The T-cell lines showed a peak response at a chemokine concentration of 10-50 ng/ml, whereas the T-cell clone responded optimally at 100 ng/ml. In contrast to a general capability of T-cells to migrate on 2-D ECM, only some of the T-cell lines were capable of 3-D migration into Matrigel or a collagen matrix. The infiltrative capacity was unrelated to the capacity to migrate on or adhere to the substrata. T-cell lines with a capacity to infiltrate produced matrix metalloproteinase-9 (MMP-9) and tissue inhibitor of matrix metalloproteinases-1 (TIMP-1), whereas non-infiltrating cell lines did not produce MMP-9. T-cell lines capable of infiltrating Matrigel or collagen responded to chemokines exposure with increased infiltration, but the chemokines did not render non-infiltrative cell lines infiltrative. Stimulation of infiltration of T-cell lines into collagen by the chemokine SDF-1α was inhibited by somatostatin, a neuropeptide with immunosuppressive properties. In conclusion, the ability to migrate on 2-D substrata and to infiltrate into 3.D substrata was found to be distinguishable properties of T cells. failure of some T-cell lines to infiltrate correlated with the lack of expression of MMP-9. Chemokines stimulated infiltration of infiltrative T-cell lines into collagen and Matrigel but did not render non-infiltrative T-cell lines infiltrative. Finally, a possible physiological mechanism for modulation of the chemokine-stimulated 3-D migration was demonstrated.</p>

Immunology

extracellular matrix

fibronectin

collagen type IV

laminin

neuropeptide

chemokine

TIMP-1

MMP-9

T cells

Migration

Immunologi

Immunology

Immunologi

Migration on extracellular matrix surface and infiltration into matrix - two distinguishable activities of human T cells

Ivanoff, Jyrki

January 2003

Migration of T-lymphocytes on a surface coated with extracellular matrix (ECM) components (two-dimensional (2-D) migration) and migration (infiltration) into a matrix (Three-dimesional (3-D) migration) are complex events and the underlying mechanisms are not yet fully understood. Here 2-D and 3-D migration were studied by use of seven leukemic T-cell lines representing discrete differentiation stages, a non-leukemic T-cell clone, and normal peripheral blood T cells. peripheral blood lymphocytes and the T-cell clone produced nanogram quantities of various chemokines, as compared to a production of ≤ 0.05 ng/ml by the T leukemia cell lines. In a Boyden chamber system, the leukemic T-cell lines showed haptotactic migration on fibronectin. The migration was augmented bu exposure to chemokines, including RANTES, MIP-1α, MIP-1β, and IL-8. The T-cell lines showed a peak response at a chemokine concentration of 10-50 ng/ml, whereas the T-cell clone responded optimally at 100 ng/ml. In contrast to a general capability of T-cells to migrate on 2-D ECM, only some of the T-cell lines were capable of 3-D migration into Matrigel or a collagen matrix. The infiltrative capacity was unrelated to the capacity to migrate on or adhere to the substrata. T-cell lines with a capacity to infiltrate produced matrix metalloproteinase-9 (MMP-9) and tissue inhibitor of matrix metalloproteinases-1 (TIMP-1), whereas non-infiltrating cell lines did not produce MMP-9. T-cell lines capable of infiltrating Matrigel or collagen responded to chemokines exposure with increased infiltration, but the chemokines did not render non-infiltrative cell lines infiltrative. Stimulation of infiltration of T-cell lines into collagen by the chemokine SDF-1α was inhibited by somatostatin, a neuropeptide with immunosuppressive properties. In conclusion, the ability to migrate on 2-D substrata and to infiltrate into 3.D substrata was found to be distinguishable properties of T cells. failure of some T-cell lines to infiltrate correlated with the lack of expression of MMP-9. Chemokines stimulated infiltration of infiltrative T-cell lines into collagen and Matrigel but did not render non-infiltrative T-cell lines infiltrative. Finally, a possible physiological mechanism for modulation of the chemokine-stimulated 3-D migration was demonstrated.

Immunology

extracellular matrix

fibronectin

collagen type IV

laminin

neuropeptide

chemokine

TIMP-1

MMP-9

T cells

Migration

Immunologi

Immunology

Immunologi

The von Hippel-Lindau protein and collagen IV alpha 2 : an insight into the mechanisms by which the von Hippel-Lindau protein regulates extracellular matrix assembly and function

Ramlal, Nishant.

January 2008

The von Hippel-Lindau (VHL) disease is a hereditary cancer syndrome that is transmitted in an autosomal dominant manner. The disease is characterized by the formation of highly angiogenic tumors in many organs but the main causes of mortality are renal cell carcinomas and hemangioblastomas. Mutations in the VHL protein are responsible for the pathogenesis of the disease. VHL associates with elongin Band C to form the VBC complex. The cullin 2 protein (CUL2) and ring box protein 1 (RBX1) also associate with the VBC complex to form an E3 ubiquitin ligase involved in the ubiquitination and subsequent degradation of the hypoxia inducible transcription factor (HIF2alpha). Mutations in VHL that abrogate its E3 ligase activity lead to increased levels ofHIF2alpha and the subsequent accumulation of pro-proliferative and pro-angiogenic HIF2alpha target genes. VHL also has an important function in the regulation of extracellular matrix (ECM) assembly which is independent of its HIF2alpha regulation pathway. VHL's regulation of ECM assembly was shown to have important consequences for tumor angiogenesis and cell invasion. It was shown to be necessary for the proper assembly of a fibronectin matrix and was most recently found to interact with collagen IV alpha 2 (COL4A2). The aim of this thesis is to further characterize the VHL-COL4A2 interaction. VHL was shown to interact directly and specifically to COL4A2 and is necessary for proper COL4A2 matrix assembly. The association of VHL with COL4A2 appears to be independent of its functions as an E3 ubiquitn ligase and CUL2 was identified as part of the VBC complex that associates with collagen IV (COL4). Furthermore, a strategy to identify the binding site of VHL on COL4A2 has been employed and is in progress. These experiments represent the beginning of investigations into the novel interaction between VHL and COL4A2.

Carcinoma, Renal Cell -- metabolism.

Extracellular Matrix -- metabolism.

Collagen Type IV -- metabolism.

The von Hippel-Lindau protein and collagen IV alpha 2 : an insight into the mechanisms by which the von Hippel-Lindau protein regulates extracellular matrix assembly and function

Ramlal, Nishant.

January 2008

No description available.

Collagen Type IV -- metabolism.

Carcinoma, Renal Cell -- metabolism.

Extracellular Matrix -- metabolism.

Investigating the role of the von Hippel Lindau protein in tumor suppression through regulation of extracellular matrix assembly

Kurban, Ghada.

January 2007

No description available.

Carcinoma, Renal Cell -- metabolism.

Extracellular Matrix -- metabolism.

Hippel-Lindau Disease -- metabolism.

Collagen Type IV -- metabolism.

Die Bedeutung des Kollagenrezeptors α2β1- Integrin bei der Pathogenese und Prävention der Nierenfibrose in hereditären Typ IV- Kollagen- Erkrankungen / The importance of the collagen- receptor integrin α2β1 in the pathogenesis and prevention of renal fibrosis in hereditary type IV collagen diseases

Martin, Maria

09 May 2011

No description available.

610 Medizin, Gesundheit

Medicine

Kollagen Typ IV

Integrin α2β1

Nierenfibrose

Glomeruläre Basalmembran

Alport- Syndrom

Alport- Mausmodell

Collagen type IV

Integrin α2β1

Renal fibrosis

Glomerular basement membrane

Alport`s syndrome

Alport mouse model

44.61

44.48

MED 418: Nephrologie