(Received for publication, September 24, 1996, and in revised form, November 18, 1996)
From the Orthopedic Research Laboratories, Department of Orthopedics, University of Washington, Seattle, Washington 98195
Fibronectin is a highly conserved dimeric glycoprotein found in high concentrations in plasma and widely distributed in low concentrations in the extracellular matrix of tissues. The protein is the product of a single gene, but multiple splicing variants are expressed that show tissue specificity. Three exons (IIIA, IIIB, and V) can be alternatively spliced to produce different fibronectin isoforms. We report here that fibronectin is a remarkably abundant component of the extracellular matrix of bovine tracheal cartilage, increasing with age to more than 20% of the tissue, dry weight. This matrix form of fibronectin is inextractable by 4 M guanidine HCl, indicating that it is a covalently cross-linked structural component. By protein sequence analysis, the main molecular form of fibronectin in bovine tracheal cartilage was shown to lack the ED-B domain encoded by exon IIIB.
Fibronectin is a widely distributed glycoprotein abundant in plasma and in small amounts in most extracellular matrices. It functions as an adhesion molecule with a key role suspected in various cellular processes including migration, morphogenesis, differentiation, and tissue repair (reviewed in Refs. 1 and 2). Evidence of altered fibronectin expression has also been reported for a range of tissues and pathologic conditions that include osteoarthritis (3-6) and rheumatoid arthritis (7-9).
The fibronectin molecule is a disulfide-bonded homodimer of 250-kDa subunits. More than 90% of the protein sequence consists of three types of repeating domains referred to as types I, II, and III homologies (10-12). Multiple forms of fibronectin result from alternative splicing of at least three exons in the primary RNA transcript of the single fibronectin gene (12-16). Two of these exons encode type III elements referred to as ED-A (exon IIIA) and ED-B (exon IIIB), which are either wholly included or excluded (17-20). The third variable region (III-CS (exon V)), can be included in total or in part (12). The pattern of fibronectin RNA splicing exhibits tissue specificity. Hepatocytes, for example, synthesize plasma fibronectin that excludes both ED-A and ED-B domains, whereas most other tissues produce cellular fibronectins that include either one or both of these domains (1, 2, 21, 22).
The extracellular matrix of cartilage consists primarily of collagens and proteoglycans with lesser amounts of non-collagenous proteins (23). Although grossly similar to articular cartilage in this respect, hyaline cartilages of the respiratory tract are distinguished by their unique profile of non-collagenous matrix proteins (23). Most prominent is cartilage matrix protein (CMP),1 a disulfide-bonded 148-kDa homotrimeric molecule first identified as a major insoluble component of mature bovine tracheal cartilage (24). Lesser amounts of CMP were present in nasal septum and in auricular, epiphyseal, and xiphisternal cartilages (25).
In attempting to define the mechanism of CMP cross-linking in tracheal cartilage, we found that fibronectin is also a major structural component of the extracellular matrix, reaching 20% or more of the tissue, dry weight, in older animals. From sequence analysis of fibronectin fragments extracted proteolytically from the tissue, we also show that the predominant fibronectin isoform in bovine tracheal cartilage lacks the ED-B domain.
Bovine tracheae from
cattle of three age groups (calf, 2-year, and 5-year animals) were
obtained at slaughter and immediately frozen and stored at 20 °C
prior to analysis. Soft tissue and perichondrium were carefully
removed, and the individual tracheal rings were minced on ice, ground
to a fine powder under liquid nitrogen (Spex mill), and then extracted
with 4 M guanidine HCl, 0.05 M Tris-HCl, pH
7.5, at 4 °C for 24 h.
Cyanogen bromide (CNBr) and trypsin digestions were carried out on portions of the washed residue. Conditions for trypsin digestion were 1% trypsin (w/w) in 0.2 M NH4HCO3 at 37 °C for 24 h. Supernatant and washings were combined, lyophilized, and weighed, and the trypsin-insoluble residual tissue was weighed. CNBr digestion was carried out in 70% (w/v) formic acid under argon at room temperature for 24 h with a CNBr concentration of 2.5 mg CNBr/mg of tissue, dry weight (26). To separate collagenous peptides from noncollagenous peptides, the CNBr digest of bovine tracheal cartilage (20 mg) was extracted 5 times with 1 ml of 1% (v/v) trifluoroacetic acid at 60 °C for 2 min. The trifluoroacetic acid-soluble material was separated by microcentrifugation (Eppendorf). The pellet and pooled supernatants were lyophilized separately and weighed.
SDS-PAGE and Amino-terminal Sequence AnalysisBoth the trifluoroacetic acid-soluble and -insoluble components were analyzed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) (27) and also transblotted onto polyvinylidene difluoride membrane for microsequence analysis (28). Edman amino-terminal sequence analysis of phenylthiohydantoin-derivatives was performed on a gas-phase protein microsequencer (Porton 2090E) equipped with on-line high performance liquid chromatography (HPLC) analysis using the manufacturer's standard program.
Peptide ChromatographyA 47-kDa CNBr peptide of fibronectin was purified by molecular-sieve HPLC. Two columns (Toso-Haas G3000SW, 7.5 mm × 60 cm) were coupled in series and eluted with 2 M guanidine HCl, 0.05 M Tris-HCl, pH 6.8, monitoring for absorbance at 220 nm (29). The isolated peptide was desalted by dialysis and digested with endoproteinase Asp-N (sequencing grade, Boehringer Mannheim). The digest was fractionated by reverse-phase HPLC (30). Individual peptide yields were estimated from the integrated absorbance (220 nm) profile and phenylthiohydantoin-derivative recoveries on sequence analysis.
The pool of acid-insoluble material from CNBr-digested tracheal cartilage, which proved to consist primarily of non-collagenous protein fragments, increased with age for the three age groups analyzed to 57% of the digest (i.e. of the 4 M guanidine-insoluble tissue, dry weight) from a 5-year-old cow (Table I). The trypsin-soluble pool of tracheal cartilage, which was extracted without heat-denaturing the collagen in order to assess the content of non-collagenous matrix proteins by another method, also increased with age to 59% of the 4 M guanidine-insoluble dry weight. In contrast, articular cartilage from the 5-year animal yielded only 12% of its 4 M guanidine-insoluble dry weight as trypsin-soluble material when treated similarly.
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Fig. 1 compares the SDS-PAGE profiles of the
trifluoroacetic acid-soluble and trifluoroacetic acid-insoluble
fractions from CNBr-digested 5-year bovine tracheal cartilage. The
trifluoroacetic acid-soluble fraction showed the typical profile of
type II collagen CNBr peptides (Fig. 1, lane 1) (31). The identity of
each peptide band was confirmed by protein microsequencing after
blotting to polyvinylidene difluoride membrane (sequence data not
shown). The trifluoroacetic acid-insoluble material gave an
electrophoretic profile totally different from that of the acid-soluble
fraction. Protein microsequence analysis identified all the major
protein bands from 5-year tracheal cartilage as CNBr peptides of bovine fibronectin (Fig. 1). Microsequence analysis from SDS-PAGE transblots of the trypsin extract of tissue showed that all major protein bands
were tryptic peptides of either bovine fibronectin or bovine CMP (data
not shown).
Based on the recovered dry weights of the various tissue fractions and the yields of protein bands on electrophoresis estimated by their staining intensities and sequencing results, fibronectin accounted for about 20% of the total dry weight of tracheal cartilage from the 5-year animal. This conservative estimate takes into account the material initially extracted by the 4 M guanidine HCl, which for the 5-year animal was less than 10% of the tissue, dry weight, as determined by dialyzing, freeze-drying, and weighing the extract.
The 47-kDa CNBr peptide that would contain the ED-B domain (if present)
was purified by molecular-sieve HPLC (Fig. 2) and then
digested with endoproteinase Asp-N. On the basis of the digest's elution profile on reverse-phase HPLC, individual Asp-N peptides were
selected for microsequence analysis (Fig. 3).
Amino-terminal sequence results on each peak are shown in Table
II. Of particular interest is the peptide giving the
DTIIPAVPPPT sequence (Table II and peak D5 in Fig. 3).
Compared to the published cDNA-predicted sequence (11), this
peptide clearly does not contain an ED-B domain, indicating that
tracheal cartilage fibronectin lacks ED-B (Fig. 4). The
presence or absence of the other variable domain, ED-A, could not be
established from these analyses. The findings are in agreement with a
recent report demonstrating that fibronectin mRNA from canine
tracheal cartilage was 100% ED-B-negative (32).
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Fibronectin is present in normal articular cartilage in low concentration (33). The splicing pattern of fibronectin mRNA from chick cartilage is reported to change during chondrogenesis (22). In mesenchymal tissue of the developing limb of the embryo, fibronectin mRNA includes both ED-A and ED-B, but only ED-B is present later, in chick cartilage. In contrast, fibronectin mRNAs from chick muscle and tendon contain ED-A and lack ED-B, leading the authors to speculate that cartilage expresses an unusual form of fibronectin (22). Here, we clearly show at the protein level that the predominant fibronectin splicing variant in bovine tracheal cartilage lacks the ED-B domain. This may reflect the expression of a splicing variant that is peculiar to respiratory tract cartilages or that is indicative of a plasma origin.
The surprising finding is that fibronectin increases with age to account for 20% of the dry weight of tracheal cartilage in the most mature animal. At this level, fibronectin rivals type II collagen in content, and it may be the most prominent structural protein of the tissue. In combination, fibronectin and the 148-kDa cartilage matrix protein certainly exceed the mass of collagen in the older tissue. The results are consistent with previous observations on cultures of tracheal cartilage that synthesized fibronectin and deposited mostly in the matrix in contrast with articular cartilage explants, which released mostly to the medium (34). The findings are also comparable to the behavior of CMP, which was shown to increase in content in bovine tracheal cartilage with age in parallel with a decrease in the protein's extractability in 4 M guanidine HCl (35). It would appear, therefore, that both fibronectin and CMP become major structural components of adult respiratory tract cartilages. This is in sharp distinction to articular cartilage, which contains very small amounts of fibronectin and CMP.
The cross-linking mechanism responsible for the inextractability of fibronectin and CMP in mature tracheal cartilage is uncertain. However, it is well documented that transglutaminase is responsible for the covalent cross-linking of plasma fibronectin to fibrin during blood-clotting (36). A key site of transglutaminase action in plasma fibronectin has been identified as the glutamine at the third residue from the amino terminus (37). Transglutaminase will also cross-link plasma fibronectin to native type I or type III collagens in vitro (38). It seems reasonable to suspect, therefore, that fibronectin becomes cross-linked in tracheal cartilage to collagen fibrils and/or other matrix proteins through transglutaminase-mediated reactions. CMP may accumulate and become cross-linked by the same mechanism. The biological significance is unknown, but profound effects on the material properties of the tissue of such a large pool of interfibrillar protein can be expected.
We thank Kae Pierce for expert assistance in the preparation of this manuscript.
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