Multiple mechanisms of dissociated epidermal cell spreading.

To test the possibility that epidermal cells use a common basement membrane protein whenever they spread, in vitro experiments were conducted using trypsin-dissociated guinea pig epidermal cells and the following proteins: human serum, bovine serum albumin, serum fibronectin, Type IV collagen, laminin, and epibolin (a recently described serum glycoprotein which supports epidermal cell spreading; Stenn, K.S., 1981, Proc. Natl. Acad. Sci. U.S.A. 78:6907.). When the cells were added to media containing the specific proteins, all the tested proteins, except for serum albumin, supported cell spreading. Added to protein-coated substrates in defined media, the cells spread on fibronectin, epibolin, and laminin-Type IV collagen, but not on albumin or whole serum. In none of these experiments were the results qualitatively affected by the presence of cycloheximide. Antibodies to a specific protein blocked cell spreading on that protein but not on the other active proteins, e.g. whereas antibodies to epibolin blocked cell spreading on epibolin, they did not affect spreading on fibronectin, collagen, or laminin. In a second assay in which the cells were allowed to adhere to tissue culture plastic before the protein-containing medium was added, the cells spread only if the medium contained epibolin. Moreover, under these conditions the spreading activity of whole serum and plasma was neutralized by antiepibolin antibodies. These results support the conclusion that dissociated epidermal cells possess multiple spreading modes which depend, in part, on the proteins of the substrate, proteins of the medium, and the sequence of cell adhesion and protein exposure.

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Chemistry of collagen cross-links: glucose-mediated covalent cross-linking of type-IV collagen in lens capsules

Biochemical Journal ◽

10.1042/bj2960489 ◽

1993 ◽

Vol 296 (2) ◽

pp. 489-496 ◽

Cited By ~ 73

Author(s):

A J Bailey ◽

T J Sims ◽

N C Avery ◽

C A Miles

Keyword(s):

Type Iv Collagen ◽

Cross Linking ◽

Mechanical And Thermal Properties ◽

Maximum Strain ◽

Scanning Calorimetry ◽

Melting Temperatures ◽

Type Iv ◽

Collagen Molecules ◽

Cross Links

The incubation of lens capsules with glucose in vitro resulted in changes in the mechanical and thermal properties of type-IV collagen consistent with increased cross-linking. Differential scanning calorimetry (d.s.c.) of fresh lens capsules showed two major peaks at melting temperatures Tm 1 and Tm 2 at approx. 54 degrees C and 90 degrees C, which can be attributed to the denaturation of the triple helix and 7S domains respectively. Glycosylation of lens capsules in vitro for 24 weeks caused an increase in Tm 1 from 54 degrees C to 61 degrees C, while non-glycosylated, control incubated capsules increased to a Tm 1 of 57 degrees C. The higher temperature required to denature the type-IV collagen after incubation in vitro suggested increased intermolecular cross-linking. Glycosylated lens capsules were more brittle than fresh samples, breaking at a maximum strain of 36.8 +/- 1.8% compared with 75.6 +/- 6.3% for the fresh samples. The stress at maximum strain (or ‘strength’) was dramatically reduced from 12.0 to 4.7 N.mm.mg-1 after glycosylation in vitro. The increased constraints within the system leading to loss of strength and increased brittleness suggested not only the presence of more cross-links but a difference in the location of these cross-links compared with the natural lysyl-aldehyde-derived cross-links. The chemical nature of the fluorescent glucose-derived cross-link following glycosylation was determined as pentosidine, at a concentration of 1 pentosidine molecule per 600 collagen molecules after 24 weeks incubation. Pentosidine was also determined in the lens capsules obtained from uncontrolled diabetics at a level of about 1 per 100 collagen molecules. The concentration of these pentosidine cross-links is far too small to account for the observed changes in the thermal and mechanical properties following incubation in vitro, clearly indicating that another as yet undefined, but apparently more important cross-linking mechanism mediated by glucose is taking place.

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Shift in collagen type as an early response to induction of the metanephric mesenchyme.

The Journal of Cell Biology ◽

10.1083/jcb.89.2.276 ◽

1981 ◽

Vol 89 (2) ◽

pp. 276-283 ◽

Cited By ~ 80

Author(s):

P Ekblom ◽

E Lehtonen ◽

L Saxén ◽

R Timpl

Keyword(s):

Basal Lamina ◽

Type Iv Collagen ◽

Early Response ◽

Type I ◽

Metanephric Mesenchyme ◽

Type Iv ◽

Interstitial Collagens ◽

Membrane Components

Conversion of the nephrogenic mesenchyme into epithelial tubules requires an inductive stimulus from the ureter bud. Here we show with immunofluorescence techniques that the undifferentiated mesenchyme before induction expresses uniformly type I and type III collagens. Induction both in vivo and in vitro leads to a loss of these proteins and to the appearance of basement membrane components including type IV collagen. This change correlates both spatially and temporally with the determination of the mesenchyme and precedes and morphological events. During morphogenesis, type IV collagen concentrates at the borders of the developing tubular structures where, by electron microscopy, a thin, often discontinuous basal lamina was seen to cover the first pretubular cell aggregates. Subsequently, the differentiating tubules were surrounded by a well-developed basal lamina. No loss of the interstitial collagens was seen in the metanephric mesenchyme when brought into contact with noninducing tissues or when cultured alone. Similar observations were made with nonnephrogenic mesenchyme (salivary, lung) when exposed to various heterotypic tissues known to induce tubules in the nephrogenic mesenchyme. The sequential shift in the composition of the extracellular matrix from an interstitial, mesenchymal type to a differentiated, epithelial type is so far the first detectable response of the nephrogenic mesenchyme to the tubule-inducing signal.

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Inhibition of laminin self-assembly and interaction with type IV collagen by antibodies to the terminal domain of the long arm.

The Journal of Cell Biology ◽

10.1083/jcb.103.5.1689 ◽

1986 ◽

Vol 103 (5) ◽

pp. 1689-1697 ◽

Cited By ~ 44

Author(s):

A S Charonis ◽

E C Tsilibary ◽

T Saku ◽

H Furthmayr

Keyword(s):

Self Assembly ◽

Binding Sites ◽

Type Iv Collagen ◽

Specific Interaction ◽

Basement Membranes ◽

Complex Domain ◽

Peptide Fragment ◽

Type Iv ◽

Collagen Molecules

Laminin is a major glycoprotein of the basement membrane. Although its precise localization and orientation within this structure is unknown, it is presumably anchored to other macromolecules such as type IV collagen or proteoheparan sulfate. In vitro, laminin has the ability to self-assemble and to bind to type IV collagen molecules at distinct sites. To identify more precisely the domains of the complex, cross-shaped laminin molecule that are involved in these interactions, images of laminin-laminin dimers and laminin-type IV collagen complexes obtained by the rotary shadowing method were analyzed. We observed that the complex domain at the end of the long arm of laminin is predominantly involved in these interactions. By using Fab fragments of antibodies specific for a peptide fragment derived from this complex domain, it is shown that laminin self-assembly is inhibited in their presence, as measured by turbidity and by electron microscopy. In addition, these antibodies inhibit the specific interaction of laminin with type IV collagen. These data suggest that the complex domain at the end of the long arm of laminin contains binding sites of potential importance for the assembly of basement membranes.

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In vitro and post-transplantation differentiation of human keratinocytes grown on the human type IV collagen film of a bilayered dermal substitute

Experimental Cell Research ◽

10.1016/0014-4827(91)90102-z ◽

1991 ◽

Vol 193 (2) ◽

pp. 310-319 ◽

Cited By ~ 112

Author(s):

Estelle Tinois ◽

Jerome Tiollier ◽

Martine Gaucherand ◽

Henri Dumas ◽

Michel Tardy ◽

...

Keyword(s):

Type Iv Collagen ◽

Human Keratinocytes ◽

Dermal Substitute ◽

Post Transplantation ◽

Collagen Film ◽

Human Type ◽

Type Iv

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Regulation of the RhoA pathway in human endothelial cell spreading on type IV collagen: role of calcium influx

Journal of Cell Science ◽

10.1242/jcs.112.19.3205 ◽

1999 ◽

Vol 112 (19) ◽

pp. 3205-3213 ◽

Cited By ~ 1

Author(s):

L. Masiero ◽

K.A. Lapidos ◽

I. Ambudkar ◽

E.C. Kohn

Keyword(s):

Endothelial Cells ◽

Endothelial Cell ◽

Focal Adhesion ◽

Type Iv Collagen ◽

Cell Spreading ◽

Stress Fiber ◽

Fiber Formation ◽

Stress Fibers ◽

Type Iv ◽

Stress Fiber Formation

We have shown that nonvoltage-operated Ca(2+) entry regulates human umbilical vein endothelial cell adhesion, migration, and proliferation on type IV collagen. We now demonstrate a requirement for Ca(2+) influx for activation of the RhoA pathway during endothelial cell spreading on type IV collagen. Reorganization of actin into stress fibers was complete when the cells where fully spread at 90 minutes. No actin organization into stress fibers was seen in endothelial cells plated on type I collagen, indicating a permissive effect of type IV collagen. CAI, a blocker of nonvoltage-operated Ca(2+) channels, prevented development of stress fiber formation in endothelial cells on type IV collagen. This permissive effect was augmented by Ca(2+) influx, as stimulated by 0. 5 microM thapsigargin or 0.1 microM ionomycin, yielding faster development of actin stress fibers. Ca(2+) influx and actin rearrangement in response to thapsigargin and ionomycin were abrogated by CAI. Activated, membrane-bound RhoA is a substrate for C3 exoenzyme which ADP-ribosylates and inactivates RhoA, preventing actin stress fiber formation. Pretreatment of endothelial cells with C3 exoenzyme prevented basal and thapsigargin-augmented stress fiber formation. While regulation of Ca(2+) influx did not alter RhoA translocation, it reduced in vitro ADP-ribosylation of RhoA (P(2)<0. 05), suggesting Ca(2+) influx is needed for RhoA activation during spreading on type IV collagen; no Ca(2+) regulated change in RhoA was seen in HUVECs spreading on type I collagen matrix. Blockade of Ca(2+) influx of HUVEC spread on type IV collagen also reduced tyrosine phosphorylation of p190Rho-GAP and blocked thapsigargin-enhanced binding of p190Rho-GAP to focal adhesion kinase. Thus, Ca(2+) influx is necessary for RhoA activation and for linkage of the RhoA/stress fiber cascade to the focal adhesion/focal adhesion kinase pathway during human umbilical vein endothelial cell spreading on type IV collagen.

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Retraction Note: Type IV collagen α1-chain noncollagenous domain blocks MMP-2 activation both in-vitro and in-vivo

Scientific Reports ◽

10.1038/s41598-020-76500-9 ◽

2020 ◽

Vol 10 (1) ◽

Author(s):

Yakkanti Akul Sudhakar ◽

Raj Kumar Verma ◽

Smita C. Pawar

Keyword(s):

Type Iv Collagen ◽

Link Type ◽

Type Iv

Editor's Note: this Article has been retracted; the Retraction Note is available at https://www.nature.com/articles/s41598-020-76500-9

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Immunological Identification of Organ Specific Proteins and Transcripts in Developing Barley Grains

Zeitschrift für Naturforschung C ◽

10.1515/znc-1993-7-814 ◽

1993 ◽

Vol 48 (7-8) ◽

pp. 609-615

Author(s):

Helge Klungland ◽

Marie Bosnes

Keyword(s):

Specific Protein ◽

Barley Grain ◽

Starchy Endosperm ◽

Sds Page ◽

Organ Specific ◽

Specific Proteins ◽

Barley Grains ◽

Immunological Identification

In vitro translated proteins from poly(A+)RNA of immature barley starchy endosperm and embryos were immunoadsorbed with antibodies raised against proteins of aleurone layers, starchy endosperm and embryos. Four starchy endosperm and eight embryo specific transcripts were detected. In addition, several mRNA s were restricted to only two of the three tissues.Comparing SDS-PAGE patterns of the in vivo protein extracts against which the antibodies were raised, four aleurone, six starchy endosperm and four embryo-specific protein bands were detectable. As for the in vitro translated proteins, several in vivo protein bands were here present in only two of the three tissues. Of eight known barley grain proteins for which antibodies were available, only three were present in developing embryos.

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Extracellular matrix production by cat retinal pigment epithelium in vitro: Characterization of type IV collagen synthesis

Experimental Eye Research ◽

10.1016/0014-4835(84)90167-2 ◽

1984 ◽

Vol 38 (3) ◽

pp. 291-304 ◽

Cited By ~ 19

Author(s):

Weiye Li ◽

Lawrence E. Stramm ◽

Gustavo D. Aguirre ◽

John H. Rockey

Keyword(s):

Collagen Synthesis ◽

Type Iv Collagen ◽

Pigment Epithelium ◽

Retinal Pigment ◽

Type Iv ◽

In Vitro Characterization ◽

Extracellular Matrix Production ◽

Matrix Production

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Induction of Hepatocyte Differentiation by the Extracellular Matrix and an RGD-Containing Synthetic Peptide

MRS Proceedings ◽

10.1557/proc-252-199 ◽

1991 ◽

Vol 252 ◽

Cited By ~ 16

Author(s):

David J. Mooney ◽

Robert Langer ◽

Linda K. Hansen ◽

Joseph P. Vacanti ◽

Donald E. Ingber

Keyword(s):

Extracellular Matrix ◽

Protein Secretion ◽

Synthetic Peptide ◽

Cell Spreading ◽

Specific Protein ◽

Hepatocyte Differentiation ◽

Liver Specific Protein ◽

Extensive Cell ◽

Adhesive Interactions

ABSTRACTTo design novel biomaterials for hepatocyte transplantation it will be necessary to determine whether specific extracellular matrix (ECM) molecule(s) or the adhesive interactions between the surface and hepatocytes are responsible for regulation of hepatocyte function. Purified ECM molecules (laminin, fibronectin, types I and IV collagen) and a synthetic peptide containing the arginine-glycine-aspartate (RGD) cell-binding sequence were precoated at defined densities to non-adhesive polystyrene dishes. Hepatocytes cultured on dishes coated with a low density of ECM molecules (1 ng/cm2) maintained a round morphology, and high liver-specific protein secretion rates. In contrast, culturing hepatocytes on increasing ECM densities (50–1000 ng/cm2) resulted in extensive cell spreading, a loss of liver-specific protein secretion, and cell growth. Hepatocytes cultured on dishes coated with the RGD-containing peptide did not spread even on a high density of the peptide (10,000 ng/cm2), and albumin secretion remained high for hepatocytes cultured on all peptide densities (1–10,000 ng/cm2). These results suggest that a variety of ECM molecules and synthetic peptides are capable of inducing hepatocyte differentiation in vitro, and these effects depend on their ability to promote cell spreading.

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Plumbagin Alleviates Capillarization of Hepatic Sinusoids In Vitro by Downregulating ET-1, VEGF, LN, and Type IV Collagen

BioMed Research International ◽

10.1155/2017/5603216 ◽

2017 ◽

Vol 2017 ◽

pp. 1-12

Author(s):

Guiyu Li ◽

Yue Peng ◽

Tiejian Zhao ◽

Jiyong Lin ◽

Xuelin Duan ◽

...

Keyword(s):

Liver Fibrosis ◽

Basement Membrane ◽

Molecular Mechanisms ◽

Type Iv Collagen ◽

Vascular Endothelial ◽

Liver Sinusoidal Endothelial Cells ◽

Collagen Mrna ◽

Type Iv ◽

Endothelial Growth Factor

Critical roles for liver sinusoidal endothelial cells (LSECs) in liver fibrosis have been demonstrated, while little is known regarding the underlying molecular mechanisms of drugs delivered to the LSECs. Our previous study revealed that plumbagin plays an antifibrotic role in liver fibrosis. In this study, we investigated whether plumbagin alleviates capillarization of hepatic sinusoids by downregulating endothelin-1 (ET-1), vascular endothelial growth factor (VEGF), laminin (LN), and type IV collagen on leptin-stimulated LSECs. We found that normal LSECs had mostly open fenestrae and no organized basement membrane. Leptin-stimulated LSECs showed the formation of a continuous basement membrane with few open fenestrae, which were the features of capillarization. Expression of ET-1, VEGF, LN, and type IV collagen was enhanced in leptin-stimulated LSECs. Plumbagin was used to treat leptin-stimulated LSECs. The sizes and numbers of open fenestrae were markedly decreased, and no basement membrane production was found after plumbagin administration. Plumbagin decreased the levels of ET-1, VEGF, LN, and type IV collagen in leptin-stimulated LSECs. Plumbagin promoted downregulation of ET-1, VEGF, LN, and type IV collagen mRNA. Altogether, our data reveal that plumbagin reverses capillarization of hepatic sinusoids by downregulation of ET-1, VEGF, LN, and type IV collagen.

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