SPARC, a secreted protein associated with cellular proliferation, inhibits cell spreading in vitro and exhibits Ca+2-dependent binding to the extracellular matrix.

Sage, Helene; Vernon, Robert B.; Funk, Sarah E.; Everitt, Elizabeth A.; Angello, John C.

doi:10.1083/jcb.109.1.341

Cited by 361 publications

(246 citation statements)

References 82 publications

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“…SPARC can be secreted to regulate local growth factor, ECM, and matrix metalloproteinase (MMP) activity, to modulate cell morphology and migration responses, angiogenesis, and cell proliferation and survival (Rempel et al, 2001;Francki et al, 2004;Barker et al, 2005a;Yan et al, 2005;Said et al, 2007a). In vitro, SPARC acts on many cell types as a deadhesive factor that induces cell rounding and inhibits cell migration (Sage et al, 1989b;Bradshaw and Sage, 2001), including on neuronal and glial cell lines (Ikemoto et al, 2000). However, SPARC is thought to act in vivo as a contextual regulator of cellular adhesion strength (Greenwood and Murphy-Ullrich, 1998), and is required for fibroblast migration during dermal wound healing (Basu et al, 2001), leukocyte infiltration after immune challenge (Kelly et al, 2007;Rempel et al, 2007), and tumor invasiveness (Rempel et al, 2001;Framson and Sage, 2004).…”

Section: Discussionmentioning

confidence: 99%

SPARC is expressed by macroglia and microglia in the developing and mature nervous system

Vincent

Lau

Roskams

2008

Developmental Dynamics

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SPARC (secreted protein, acidic and rich in cysteine) is a matricellular protein that is highly expressed during development, tissue remodeling, and repair. SPARC produced by olfactory ensheathing cells (OECs) can promote axon sprouting in vitro and in vivo. Here, we show that in the developing nervous system of the mouse, SPARC is expressed by radial glia, blood vessels, and other pial-derived structures during embryogenesis and postnatal development. The rostral migratory stream contains SPARC that becomes progressively restricted to the SVZ in adulthood. In the adult CNS, SPARC is enriched in specialized radial glial derivatives (Mü ller and Bergmann glia), microglia, and brainstem astrocytes. The peripheral glia, Schwann cells, and OECs express SPARC throughout development and in maturity, although it appears to be down-regulated with maturation. These data suggest that SPARC may be expressed by glia in a spatiotemporal manner consistent with a role in cell migration, neurogenesis, synaptic plasticity, and angiogenesis.

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Section: Discussionmentioning

confidence: 99%

SPARC is expressed by macroglia and microglia in the developing and mature nervous system

Vincent

Lau

Roskams

2008

Developmental Dynamics

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“…9,24 This suppression may be related to the rapid growth of tumors, since SPARC has an antiproliferative function through the modulation of cell cycle regulatory proteins or growth factors. 33 When we evaluated the relationship between SPARC suppression and clinicopathologic factors in 292 colorectal carcinomas, suppression of SPARC was not associated with age, sex, tumor site, MSI status or tumor stage. However, SPARC suppression was associated with decreased mucin production and with poor prognosis.…”

Section: Discussionmentioning

confidence: 99%

Frequent inactivation of SPARC by promoter hypermethylation in colon cancers

Yang

Kang

Koh

et al. 2007

Intl Journal of Cancer

116

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Epigenetic modification of gene expression plays an important role in the development of human cancers. The inactivation of SPARC through CpG island methylation was studied in colon cancers using oligonucleotide microarray analysis and methylation specific PCR (MSP). Gene expression of 7 colon cancer cell lines was evaluated before and after treatment with the demethylating agent 5-aza-2 0 -deoxycytidine (5Aza-dC) by oligonucleotide microarray analysis. Expression of SPARC was further examined in colon cancer cell lines and primary colorectal cancers, and the methylation status of the SPARC promoter was determined by MSP. SPARC expression was undetectable in 5 of 7 (71%) colorectal cancer cell lines. Induction of SPARC was demonstrated after treatment with the demethylating agent 5Aza-dC in 5 of the 7 cell lines. We examined the methylation status of the CpG island of SPARC in 7 colon cancer cell lines and in 20 test set of colon cancer tissues. MSP demonstrated hypermethylation of the CpG island of SPARC in 6 of 7 cell lines and in all 20 primary colon cancers, when compared with only 3 of 20 normal colon mucosa. Immunohistochemical analysis showed that SPARC expression was downregulated or absent in 17 of 20 colon cancers. A survival analysis of 292 validation set of colorectal carcinoma patients revealed a poorer prognosis for patients lacking SPARC expression than for patients with normal SPARC expression (56.79% vs. 75.83% 5-year survival rate, p 5 0.0014). The results indicate that epigenetic gene silencing of SPARC is frequent in colon cancers, and that inactivation of SPARC is related to rapid progression of colon cancers. ' 2007 Wiley-Liss, Inc.

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“…Rat bone sialoprotein cDNA (a gift of Dr. Jaro Sodek, University of Toronto) was subcloned and transcribed similarly. Intact mouse SPARC protein was isolated from the conditioned medium of PYS-2 cells and was purified as previously described (Sage et al 1989). This protein preparation was shown to disrupt barrier function in cultured endothelial cells, as described by Goldblum et al (1994), and to inhibit endothelial and smooth muscle cell proliferation in vitro, according to Funk and Sage (1993).…”

Section: Sparc Rna and Proteinmentioning

confidence: 99%

“…Ectopic expression of SPARC produced comparable muscle defects in C. elegans (Schwarzbauer and Spencer 1993). Although the precise functions of SPARC during early embryonic development are not known, a variety of potential functions have been described for SPARC in vitro, e.g., inhibition of cell-substratum adhesion and cell spreading (Sage et al 1989), binding to and/or modulation of growth factors (Hasselaar and Sage 1992;Raines et al 1992), regulation of cell cycle progression Sage 1991, 1993), and augmentation of interendothelial cell permeability (Goldblum et al 1994; reviewed in Lane and Sage 1994). Furthermore, SPARC interacts with several ECM macromolecules in vitro (Tremble et al 1993;Kelm and Mann 1991).…”

mentioning

confidence: 99%

Ectopic Expression of SPARC inXenopusEmbryos Interferes with Tissue Morphogenesis: Identification of a Bioactive Sequence in the C-terminal EF Hand

Damjanovski

Karp

Funk

et al. 1997

J Histochem Cytochem.

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SUMMARY SPARC is a matricellular Ca 2 ϩ -binding glycoprotein that exhibits both counteradhesive and antiproliferative effects on cultured cells. It is secreted by cells of various tissues as a consequence of morphogenesis, response to injury, and cyclic renewal and/or repair. In an earlier study with Xenopus embryos we had shown a highly specific and regulated pattern of SPARC expression. We now show that ectopic expression of SPARC before its normal embryonic activation produces severe anomalies, some of which are consistent with the functions of SPARC proposed from studies in vitro. Microinjection of SPARC RNA, protein, and peptides into Xenopus embryos before endogenous embryonic expression generated different but overlapping phenotypes. (a) Injection of SPARC RNA into one cell of a two-cell embryo resulted in a range of unilateral defects. (b) Precocious exposure of embryos to SPARC by microinjection of protein into the blastocoel cavity was associated with certain axial defects comparable to those obtained with SPARC RNA. (c) SPARC peptides containing follistatin-like and copper-binding sequences were without obvious effect, whereas SPARC peptide 4.2, corresponding to a disulfide-bonded, Ca 2 ϩ -binding domain, was associated with a reduction in axial structures that led eventually to complete ventralization of the embryos. Histological analysis of ventralized embryos indicated that the morphogenetic events associated with gastrulation might have been inhibited. Microinjection of other Ca 2 ϩ -binding glycoproteins, such as osteopontin and bone sialoprotein, resulted in phenotypes that were unique. We probed further the structural correlates of this region of SPARC in the context of tissue development. Co-injection of peptide 4.2 with Ca 2 ϩ or EGTA, and injection of peptide 4.2K (containing a mutated consensus Ca 2 ϩ -binding sequence), demonstrated that the developmental defects associated with peptide 4.2 were independent of Ca 2 ϩ . However, the disulfide bridge in this region of SPARC was found to be critical, as injection of peptide 4.2AA, a mutant lacking the cystine, generated no axial defects. We have therefore shown for the first time in vivo that the temporally inappropriate presence of SPARC is associated with perturbations in tissue morphogenesis. Moreover, we have identified at least one bioactive region of SPARC as the C-terminal disulfide-bonded, Ca 2 ϩ -binding loop that was previously shown to be both counteradhesive and growth-inhibitory. (J Histochem Cytochem 45:643-655, 1997) E xtracellular matrix glycoproteins make major morphoregulatory contributions to early embryonic development. Their complex, transient expression patterns, structural heterogeneity, and functional diversity indicate important roles in the modulation of a broad spectrum of cellular activities, such as adhesion, migration, communication, and/or proliferation. For example, the blastocoel roof of amphibian embryos is coated with an elaborate network of fibronectin fibers before the involution of mesodermal cells durin...

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SPARC, a secreted protein associated with cellular proliferation, inhibits cell spreading in vitro and exhibits Ca+2-dependent binding to the extracellular matrix.

Cited by 361 publications

References 82 publications

SPARC is expressed by macroglia and microglia in the developing and mature nervous system

SPARC is expressed by macroglia and microglia in the developing and mature nervous system

Frequent inactivation of SPARC by promoter hypermethylation in colon cancers

Ectopic Expression of SPARC inXenopusEmbryos Interferes with Tissue Morphogenesis: Identification of a Bioactive Sequence in the C-terminal EF Hand

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