Cablin: a novel protein of the capillary basal lamina

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Cablin: a novel protein of the capillary basal lamina

Audra J. Charron¹, Weimin Xu², Robert L. Bacallao², and Angela Wandinger-Ness³

¹ Integrated Graduate Program in the Life Sciences, Northwestern University Medical School, Chicago, Illinois 60611; ² Department of Medicine, Indiana University Medical Center, Indianapolis, Indiana 46202; and ³ Department of Pathology, University of New Mexico Health Sciences Center, Albuquerque, New Mexico 87131

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The microvascular wall is remarkably simple, consisting only of the endothelial lining, subjacent basal lamina, and underlyingperiendothelial cells. This study describes the characterizationof a novel microvascular protein. This 80,000-molecular weightprotein was predominantly associated with electron-lucent amorphousmaterial in capillary basal laminae and therefore termed cablin(protein of the capillary basal lamina). Consistent with its immunolocalizationto the microvasculature, cablin was synthesized and secreted bycultured endothelial cells and vascular smooth muscle cells. Furthermore,cablin expression was induced during neovascularization. The predictedamino acid sequence of cablin revealed a prevalence of polar aminoacids. Accounting for the low yet significant homology to several $alpha$ -helical proteins, these residues were best accommodated by secondarystructure predictions that aligned the molecule into two large $alpha$ -helical domains. The presence of the integrin-binding RGD tripeptideand a putative elastin-binding sequence suggest that this rodlikemolecule is suited to cross-link cells and matrix constituents.In this capacity it could contribute to the mechanical strengthor the angiogenic potential of themicrovasculature.

vascular smooth muscle; endothelial cell; microvascular; extracellular matrix

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

BY VIRTUE of their unique ultrastructure, microvascular beds, composed of precapillary arterioles, capillaries, and postcapillaryvenules, are the principal sites of neovascularization (7,24) and molecular exchange between the blood and the interstitialfluid (47). Because capillaries lack both a muscular wall andelaborate elastic subendothelial layers, the walls of these vesselsconsist only of the single layer of endothelial cells lining thelumen and a minimal subendothelial basal lamina (15). It isthis basal lamina and surrounding periendothelial cells that providethe capillary with mechanical support (48). Microvascular bedssuch as the renal glomerular capillaries are especially dependenton the subendothelial basal lamina for tensile strength due tothe high hydrostatic pressure experienced during the formationof plasma filtrate (10). Organized immediately subjacent tothe capillary endothelium, the basal lamina consists of a meshworkof molecules that ensheath the endothelial and periendothelialcells (46). The intimate association among endothelium, basallamina, and periendothelium facilitates rapid transport of moleculesand provides a means of intercellular and intrasystemiccommunication.

Endothelial and periendothelial cells are the primary cellular constituents of the microvasculature. The continuous endothelialcell lining of the capillary lumen acts as the primary selectivebarrier, the tightness of which directly affects vessel wall permeability(43). Subsequently, capillary periendothelial cells ("pericytes")together with the basal lamina act as a molecular sieve that limitsaccess to the interstitium (6). Pericytes and capillary endothelialcells act in concert to secrete and organize the basal laminathat forms such an integral component of capillary architecture(8, 13, 20, 23, 27, 30, 53, 55, 57).

Microvascular basal laminae, similar to those of larger muscular and elastic vessels, consist of a heterogeneous network ofextracellular matrix proteoglycans and proteins. These moleculesare integral components of the vascular architecture as well asregulators of cellular processes. Among the most thoroughly characterizedcapillary basal laminae are the renal glomerular basement membraneand the juxtaglomerular mesangial matrix (5, 14, 33, 40).A prominent constituent of these and other vascular matrices arethe microfibrils, morphologically unique 10- to 12-nm diameterfibers (34) that occupy an amorphous, electron-lucent basallamina region (7, 24). The necessity for properly assembledmicrofibrils is punctuated by the incidence of diseases in whicha single allele of a microfibrillar component is mutated. Suchdisorders include Marfan's syndrome and congenital contracturalarachnodactyly and are manifested as vascular and connective tissueabnormalities (12, 45). Microfibrils may also function asa repository for soluble effectors. For example, latent transforminggrowth factor- $beta$ (TGF- $beta$ ) binding proteins are associated with microfibrils,where TGF- $beta$ may be stored before activation (21, 38, 42).Likewise, the clotting factor thrombospondin has been localizedto microfibrils in the vascular basement membrane, where it maymediate thrombogenesis in response to vascular injury (3).A subset of capillary basal lamina proteins bind select cell-surfaceintegrins, thereby mediating cell-extracellular matrix adhesion(9-11). Integrins are heterodimeric, membrane-spanning receptorsthat serve as a molecular interface between the extra- and intracellularenvironment (2). Intracellularly, activation of signaling cascadesin response to integrin ligation serves to modulate cell motility,gene expression, and differentiation state (29). Extracellularly,integrins impact adhesion to components of the extracellular milieuin response to cellular cues (29). It is precisely this biochemicalcomplexity of capillary basal laminae that underlies their vitalfunctions in structural support, cell-extracellular matrix interactions,and metaboliteexchange.

The extracellular matrix also serves as a source of cues promoting angiogenesis and differentiation of the microvasculature.The spatiotemporal regulation of angiogenesis from existing capillaryvessels is dependent on changes in the composition and organizationof the extracellular matrix (51). The presence of appropriategrowth factors and extracellular matrix constituents dictate bothcapillary sprouting and endothelial migration through the activationof discrete signaling cascades (50, 54). Until needed, someof these growth factors are maintained in an inactive state bysequestration within matrices. For example, following capillaryinjury fibroblast growth factor is immediately released from proteoglycansto potentiate angiogenesis and promote rapid wound healing (16).Capillary endothelial cells undergoing angiogenic migration secreteboth extracellular matrix proteins and chemoattractants (51).These molecules in turn elicit the recruitment of interstitialfibroblasts and their subsequent differentiation into pericytes(49, 50). Given the developing scenario it is tempting topostulate that the cells comprising capillaries are expresslyadapted to the synthesis of a unique basal lamina that supportsboth molecular exchange andangiogenesis.

Vascular transitions to and from the highly anastomosing capillary beds are delineated by gradual modulations in vessel architectureand cellular phenotype (19, 47). The diversity of endothelialand periendothelial cells along the vasculature is thought torepresent a continuum of cellular differentiation states (49),as well as heterogeneity brought about by local demands (51).The recent discovery of proteins expressed exclusively by eithervenous or arterial endothelial cells, considered together withthe morphological diversity of these cells, provides evidenceof genetically determined distinctions between the cellular constituentsof the circulation (1, 59). The interdependence between cellulardifferentiation and extracellular matrix constituents makes itplausible that the observed biochemical and morphological gradationsare accompanied by changes in the molecular composition of microvascularbasal laminae. Whereas the inventory of the microfibrillar andintegrin-binding extracellular matrix proteins found in the basallaminae of capillaries and other vessels continues to grow, itis still incomplete. Furthermore, the identification of thosemolecular constituents selectively enriched in the microvascularwall remains a challenge. This study describes the first suchcandidate, a novel protein preferentially expressed in microvascularextracellularmatrices.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Reagents. Sodium dodecylsulfate, Triton X-100, Tween 20, AEBSF [4-(2-aminoethyl)benzenesulfonylfluoride, HCl], and Mowiolwere obtained from Calbiochem (San Diego, CA). Affigel-10 activatedresin was obtained from Bio-Rad (Hercules, CA). Horseradish peroxidase(HRP)-conjugated secondary antibodies and nitrocellulose membraneswere supplied by Amersham (Arlington Heights, IL). Super SignalECL was purchased from Pierce (Rockford, IL). FITC- and rhodamine-conjugateddonkey anti-rabbit IgG, goat anti-mouse IgG, and alkaline phosphatase-conjugatedgoat anti-rabbit IgG were supplied by Jackson ImmunoResearch (WestGrove, PA). Gold-conjugated (20 nm) goat anti-rabbit IgG, LR Whiteembedding resin, uranyl acetate, lead citrate, and nickel gridswere purchased from Ted Pella (Redding, CA). A mouse monoclonalantibody (A028) directed against an endothelial cell surface markerwas obtained from Telios Pharmaceuticals (San Diego, CA) in theform of ascites. All other chemicals and reagents were purchasedfrom Sigma (St. Louis,MO).

Isolation and characterization of cDNA. An oligo(dT)-primed $lambda$ -ZAP human placental cDNA library (3 × 10¹⁰ independent clones) was obtained from Stratagene (La Jolla, CA).The library was plated onto Escherichia coli XL-1 Blue (Stratagene)lawns and grown at 42°C for 3.5 h. Nitrocellulose filters impregnatedwith 10 mM isopropylthio- $beta$ -D-galactopyranoside were applied tothe agar plates and incubated at 37°C for an additional 3.5 h.The filters were removed and washed in Tris-buffered saline (TBS,50 mM Tris · HCl, pH 8.0, 200 mM NaCl), and nonspecific bindingsites were blocked for 1 h with TBS-T (TBS, 0.1% Tween 20) containing0.2% newborn calf serum. Antiserum directed against a unique peptide(AVWPTRTQGPLPSSLGK) or affinity-purified antipeptide antibodies(preadsorbed against E. coli lysate) were diluted in TBS-T containing0.2% newborn calf serum and incubated with the membranes for 30min at room temperature under continuous agitation. The membraneswere washed five times with TBS-T (5 min each) at room temperature.After the washes, the membranes were incubated with alkaline phosphatase-conjugatedgoat anti-rabbit IgG diluted in TBS-T containing 0.2% newborncalf serum for 30 min at room temperature. After being washedwith TBS-T (five times, 5 min each), positive plaques were identifiedusing nitroblue tetrazolium (0.05%) and bromo-chloro-indolylphosphate(0.015%) in TBS. Membranes were aligned with the agar plates andpositive plaques were isolated by suspending core samples fromthe agar plates in 1 ml of 50 mM Tris · HCl, pH 7.5, containing100 mM NaCl, 2 mM MgSO₄, 0.01% gelatin, and 3% chloroform. XL-1Blue cells were grown to OD₆₀₀ = 1.0, mixed with isolated Bluescriptphagemid stock and ExAssist helper phage (Stratagene). The cellswere incubated for 15 min at 37°C, additional media were addedto the infected cells, and the mixture was incubated at 37°C foran additional 2 h. Cells were pelleted by centrifugation for 15min at 2,000 g. The supernatant was collected, heated at 70°C,and cleared by centrifugation for 15 min at 4,000 g. The supernatantcontaining filamentous phage was collected and used to infectE. coli strain SOLR cells (Stratagene). Isolated colonies wereselected on ampicillin plates, and plasmids were isolated withthe QIAprep Miniprep kit (Qiagen, Valencia,CA).

Plasmid inserts were sequenced using the GIBCO BRL Life Technologies (Gaithersburg, MD) cycle sequencing kit. Sequence analysisof all isolated clones resulted in the identification of 10 cDNAclones, 4 of which were identical (termed c4) and chosen for sequenceanalysis. Sequencing primers were supplied by Operon (Alameda,CA). Forward primers corresponded to T3 promotor sequences containedwithin pBluescript (5'-AATTAACCCTCACTAAAGGG-3') and bases 166-193,375-394, and 444-466 of the c4 cDNA. Reverse primers correspondedto T7 promotor sequences contained within pBluescript (5'-GTAATACGACTCACTATAGGGC-3')and bases 1550-1567 of the c4 cDNA. PCR constructs encoding centralportions of the c4 cDNA (either from bases 444-1567 or from bases580-1176) were used to sequence these regions using the T3 andT7 primers (see above). Primers were end-labeled using T4 kinasewith [ $gamma$ -³³P]ATP (2-4 Ci/mol) (NEN Life Sciences Products, Boston, MA) (52).The dideoxy sequencing reactions were performed as per the manufacturer'sdirections. Sequencing gels were run on a Genomyx LR ProgrammableDNA sequencing apparatus (Genomyx, Fullerton, CA) maintained at65°C. Sequence analyses were performed using the GCG softwarepackage (Wisconsin software package version 10, Genetics ComputerGroup, Madison,WI).

Northern blotting. A 1340-bp probe corresponding to the 5' region of cablin cDNA was labeled by random priming (52). Theapproximate size and tissue expression of cablin mRNA was determinedby hybridization of the radioactive probe to a multiple tissueNorthern blot (Clontech, Palo Alto, CA) loaded with 2 µg of poly(A)⁺ mRNA per lane using ExpressHyb solution (Clonetech) and followingthe manufacturer's recommended protocol. As a control for RNAloading, the same blot was subsequently probed with a 1200-bpprobe for rat glyceraldehyde-3-phosphate dehydrogenase (18).

Recombinant protein expression and purification. The cablin cDNA insert was subcloned into pET21b (Novagen, Madison, WI) andused to express the encoded protein in E. coli strain BL-21/DE3(Stratagene) (58). The detergent-insoluble material remainingafter bacterial lysis was solubilized in 8 M urea for 1 h at roomtemperature and dialyzed successively against six changes of 50mM Tris · HCl, pH 8.0, 50 mM NaCl, and 1 mM EDTA containing decreasingconcentrations of urea. The dialysate was assayed for purity bySDS-PAGE followed by Coomassie stain, and the pure protein wasdiluted in phosphate-buffered saline (PBS) and injected (200 µg/injection)into rabbits for antibody production (Covance, Denver, PA). Freund'scomplete adjuvant was used for the primary injection, and Freund'sincomplete adjuvant was used for all subsequent boosterinjections.

Affinity purification of antibodies. Recombinant protein was dialyzed against two changes of PBS and coupled to Affigel-10resin according to manufacturer's directions. Immune rabbit serumwas bound to the resin-bound antigen and specific antibodies elutedfrom the column using standard procedures (25).

Cell culture and extract preparation. Normal human aortic smooth muscle cells, human lung microvascular endothelial cells,and human umbilical cord vein endothelial cells and their definedmedia were purchased from Clonetics (San Diego, CA). Cells wereseeded at 3,500 cells/cm² and allowed to grow to confluence over 3 days in a humidifiedatmosphere of 5% CO₂ at 37°C. Serum-free medium was added to confluentcultures and collected after 18 h. Medium from one 35-mm dishwas concentrated 10-fold and mixed with SDS-PAGE sample buffercontaining dithiothreitol. Cells were rinsed briefly in PBS, scrapedfrom the dish, and pelleted by centrifugation at 700 g for 5 min.The cell pellet was resuspended in sample buffer, sonicated for30 s, and boiled for 5 min before being loaded ontogels.

Preparation of tissue extracts. A 0.5-g sample of normal human kidney cortex was thawed from $-$ 80°C and minced on ice. Thetissue was further homogenized in 15 mM Tris · HCl, pH 8.0, and1 µM AEBSF with a Tissue Tearor (BioSpec Products, Bartlesville,OK) until completely liquefied. The homogenate was clarified bycentrifugation for 10 min at 10,000 g at 4°C. The pellet fractionwas resuspended in 5 ml of 10 mM Tris · HCl, pH 8.0, 2% SDS, 2%TX100, 10 mM EDTA, 0.5 M NaCl, 50 mM dithiothreitol, 1 µM AEBSF,and 1 µM CLAP (chymostatin, leupeptin, antipain, and pepstatinA), and incubated at 4°C for 8 h while being rocked. The extractedpellet was again subjected to centrifugation, and the resultingsupernatant fraction was filtered through a 0.4-µm syringe filter,SDS-PAGE sample buffer was added, and the fraction was treatedwith 63 mM iodoacetamide (added as a solid) for 30 min at roomtemperature in thedark.

SDS-PAGE and Western blot analysis. Proteins were separated on 10% SDS-PAGE gels. After electrophoresis, gels were transferredto nitrocellulose membranes. Nonspecific binding sites on immunoblotswere blocked by a 1-h incubation period at room temperature with0.5% nonfat dried milk in TBS-T. Blots were probed with 1 µg/mlof primary antibody (in some cases preincubated with a 10-foldmolar excess of immunogen) followed by 1 µg/ml of HRP-conjugatedsecondary antibodies. Bound HRP-conjugated antibodies were detectedusing SuperSignal ECL reagent. Control blots were probed withpreimmune serum and never gave anysignal.

Angiogenesis model. Hypoxia-induced neovascularization was incited by following established experimental procedures (56).Briefly, mice were placed in a hyperoxic environment of 75% oxygenfrom postnatal days 7-12. From postnatal days 12-17 mice werereturned to atmospheric oxygen (a hypoxic environment relativeto 75% oxygen), after which time they were euthanized. Eyes wereenucleated, embedded in OCT compound, and 10-µm frozen sectionscut for immunohistochemicalanalysis.

Immunofluorescence microscopy. Unfixed frozen tissue sections embedded in OCT were cut (5-10 µm in thickness) and collectedon Probe-On Plus microscope slides (Fisher Scientific, Chicago,IL). Sections were blocked with PBS containing 0.2% cold waterfish skin gelatin for 30 min at room temperature before incubationwith antibodies. Sections were incubated with either affinity-purifiedantibodies, immune serum, or preimmune serum at a concentrationof 10 µg/ml for 1 h at 37°C. Primary antibodies were detectedwith FITC- or rhodamine-conjugated goat anti-rabbit IgG or goatanti-mouse IgG (20 µg/ml), and sections were mounted in Mowiol4-88 or Vectashield-DAPI (Vector, Burlingame, CA). No signal wasobserved in sections stained with preimmune serum. Images werecollected using an inverted Zeiss LSM 410 or Biorad MRC600, bothequipped with He-Ne and Ar-Krlasers.

Histological staining. Sections were stained with Mayer's hematoxylin and counter-stained with eosin (Sigma) according tomanufacturer's instructions. Elastic fibers in bovine mitral valvewall were visualized by staining sections with a 1/10 aqueoussolution of India ink for 3 min, followed by extensive rinsingwithwater.

Immunoelectron microscopy. A normal kidney from a Sprague-Dawley male rat was excised immediately after decapitation and choppedinto 0.5-mm² pieces in 0.1 M sodium cacodylate, 2.5% glutaraldehyde, 2% paraformaldehyde,and incubated in this fixative for 2 h at room temperature. Reactivealdehyde groups were quenched with 50 mM ammonium chloride in0.1 M sodium cacodylate for 30 min at room temperature. The tissuewas then extracted for 30 min at room temperature with 0.1% saponinin 0.1 M sodium cacodylate then rinsed briefly in this bufferalone. The tissue was dehydrated by successive incubations (5min each at room temperature) in 10%, 30%, and 50% ethanol followedby two incubations (30 min each at room temperature) in 70% ethanol.The minced pieces were embedded in LR White resin according tomanufacturer's instructions. Sections (60- to 70-nm-thick) werecut from the polymerized blocks and collected on Formvar-coatednickel grids. Sections were immunolabelled by floating them upsidedown on drops of primary antibody diluted to 10 µg/ml in PBS containing0.2% cold water fish skin gelatin for 1 h at room temperature,rinsing several times in PBS, and incubating for 30 min at roomtemperature with 20-nm gold-conjugated goat anti-rabbit IgG diluted1/50 in PBS, 0.2% fish skin gelatin. Rinsed sections were thencontrasted sequentially with uranyl acetate and lead citrate.Immunogold decoration was not evident when sections were incubatedwith preimmune serum. Images were collected using a Hitachi H-600transmission electronmicroscope.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Isolation and characterization of a cDNA clone encoding a novel protein. The screening of an oligo(dT)-primed human placentalexpression cDNA library with an antibody directed against a uniquepeptide (see MATERIALS AND METHODS) resulted in four independentisolates, termed c4, containing identical 1.742-kb inserts. Thenucleotide and deduced amino acid sequences (Fig. 1A) encodedby the 1.742-kb cDNA were found to represent a previously uncharacterizedmolecule based on searches of both nucleotide and protein databases.Evident in the sequence was a single, long, open reading frameof 270 amino acids, a polyadenylation signal (AATAAA), and a poly(A)tail. The lack of a consensus sequence for translation initiation(31) suggested that c4 most likely encoded the carboxy terminusof a novel protein. Searches of both the expressed sequence tagdatabase and nonredundant nucleotide databases identified severalentries matching the sequence of c4, but none provided any additional5' sequence information.

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Fig. 1. A novel protein encoded by c4. A: partial nucleotide sequence and deduced amino acid sequence from the open reading frame are shown. Numbers refer to positions of nucleotides (top) or amino acids (bottom). A putative elastin binding sequence is underlined. Integrin recognition motif RGD sequence is shown in bold. * Stop codon position. B: secondary structure of protein was predicted using the Plotstructure function of the GCG Software Package. Hydrophilicity predictions were made according to Kyte-Doolittle, whereas turns, $alpha$ -helical regions, and $beta$ -sheets were predicted according to Garnier-Osguthorpe-Robson. N-linked glycosylation sites (N-linked) were not present in this portion of the protein.

Both the deduced amino acid composition and primary structure of the c4 protein indicate that it is likely to be an $alpha$ -helicalmolecule (Fig. 1). The predominance of glutamic acid, alanine,and leucine residues found throughout the c4 protein (Fig. 1A)is not unusual in $alpha$ -helical proteins. Appropriate spacing of chargedand polar side chains lends stability to $alpha$ -helices through theformation of salt bridges (35), whereas alanine residues oftenconstitute the hydrophobic face of helices (4, 36). Structureprediction algorithms configured the c4 protein into two long $alpha$ -helical regions separated by turns (Fig. 1B). Contained withinthe protein is a 60 amino acid sequence with 22% homology to amicrofibrillar elastin-binding peptide (underlined in Fig. 1A)(44). Also apparent is the tripeptide sequence RGD, known tomediate binding to the integrin family of cell adhesion molecules(bold letters in Fig. 1A). The carboxy terminus of the proteincontains numerous prolines and is expected to form a rigid tailon the end of this predicted helical molecule. The absence ofa contiguous stretch of hydrophobic amino acids suggests thatthe c4 protein lacks a membrane-spanningdomain.

Comparison of the deduced amino acid sequence to known proteins revealed significant homologies to several structural proteinspossessing $alpha$ -helical and coiled-coil domains. Among those withover 20% identity were the hemidesmosomal protein plectin, thebacterial import protein TolA, protein A kinase anchoring protein,and nonmuscle myosin heavy chain II. Without exception, homologywith the c4 protein was limited to the glutamic acid-alanine-leucine-rich $alpha$ -helical domains of these proteins, implying that these primaryamino acid sequences mediate folding into similar domains in functionallydiverse proteins. These data are suggestive that the c4 proteinexists as a rod-shaped or coiled-coilmolecule.

Tissue-specific expression of the full-length c4 transcript. The distribution of the full-length c4 transcript in a panelof human tissues was determined by Northern blot analysis (Fig.2). A c4 probe hybridized with a single transcript of ~2.5 kbin all tissues tested. The message was most abundant in placenta(Pl), pancreas (Pa), kidney (K), and skeletal muscle (M), whereaslittle was detected in the brain (B). Moderate expression wasdetected in the heart (H). These data indicate that c4 encodesa protein, which is expressed in a variety of tissue types. Aprobe for glyceraldehyde-3-phosphate dehydrogenase was used asa control for RNA loading and as expected a transcript of 1.26kb was detected in all lanes but was most abundant in heart andskeletal muscle samples (Fig. 2, bottom panel).

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Fig. 2. c4 mRNA is detected in various tissues by Northern blot analysis. Top panel: a multitissue human poly(A)⁺ RNA blot with 2 µg RNA/lane was hybridized to a 1340-bp probe corresponding to 5' region of the c4 cDNA. H, heart; B, brain; Pl, placenta; Lu, lung; Li, liver; M, skeletal muscle; K, kidney; Pa, pancreas. Position of molecular size markers is as shown. Bottom panel: same blot reprobed with a rat GAPDH probe. Hybridization of both radioactive probes was detected after an overnight exposure to X-ray film at $-$ 80°C with an intensifying screen.

An 80,000-molecular weight protein is the product of c4 in vivo. Western blot analysis was used to analyze the molecular weightand the predicted tissue distribution of the protein encoded byc4. Polyclonal antibodies generated against purified recombinantprotein encoded by c4 were used to probe an immunoblot of normalhuman kidney tissue extracts (Fig. 3). Both the antiserum (lane1) and the affinity-purified antibodies (lane 3) identified aprotein of 80,000 molecular weight, whereas the preimmune serum(lane 2) and immune serum preincubated with immunizing antigen(lane 4) failed to bind the immunoblot. Tissue extracts from mitralvalve wall and pancreas were also found to contain this 80,000-molecularweight protein (data not shown). Thus the polyclonal antibodyvery specifically recognized an 80,000-molecular weight proteinin tissue extracts expressing the c4 transcript. Efforts werenext focused on immunolocalization of the antigen in situ.

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Fig. 3. c4 encodes an 80,000-molecular weight protein. Tissue extracts were resolved by preparative gel SDS-PAGE and transferred to a nitrocellulose membrane. Individual strips containing 10 µg of total protein were cut and probed with lane 1, immune serum; lane 2, preimmune serum; lane 3, an affinity-purified antibody directed against recombinant c4 protein; or lane 4, same affinity-purified antibody preincubated with a 100-fold excess of immunizing antigen. Antibody binding was visualized using a horseradish peroxidase-conjugated secondary antibody and chemiluminescent substrate. Strips were carefully realigned before exposure to X-ray film. Relative migration of molecular weight standards is as indicated.

Localization of c4 protein to the vasculature. Immunofluorescence microscopy was utilized to examine the localization of thec4 protein in human kidney cortex, bovine mitral valve wall, andrat pancreas. An abundance of the protein was evidenced in thekidney cortex (Fig. 4, A and D), where it was specifically limitedto the glomeruli and small (4-15 µm diameter) peritubular vessels(Fig. 4A, arrow; see also Fig. 5). Examination of mitral valvewall, a relatively homogeneous tissue consisting of the endotheliumand vascular basement membrane, revealed staining of discretecurvilinear fibers oriented parallel to the direction of bloodflow (Fig. 4, B and E). Furthermore, the immunostaining in a sectionof pancreatic tissue enriched in elastic and muscular vesselswas also restricted to the vasculature (Fig. 4, C and F). Theseresults demonstrated that the c4 protein was expressed in thevasculature, predominantly in small vessels.

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Fig. 4. c4 Protein is present in the vasculature. Thin sections of human kidney (A), bovine mitral valve wall (B), and rat pancreas (C) were stained with polyclonal antibody directed against recombinant c4 protein and visualized with a rhodamine-conjugated secondary antibody. D: hematoxylin-eosin stained section of kidney similar to that in A was visualized with brightfield microscopy. E and F: after immunofluorescence imaging, sections were stained with India ink (E) to visualize elastic fibrils or hematoxylin-eosin (F), focal fields were relocated, and tissue components visualized with brightfield microscopy. Arrows, peritubular capillaries; g, glomeruli; l, vascular lumen; a, arteriole. Magnifications: A, C, and D, ×400; B and E, ×630; F, ×350.

Antibodies to the c4 protein specifically stain microvascular elements. Double immunofluorescence studies were employed todefinitively identify the vascular elements with which the 80,000-molecularweight protein was preferentially associated. Monoclonal antibodyA028, directed against an unspecified endothelial cell surfaceprotein, was used to visualize all vascular structures. Immunostainingof kidney tissue with this antibody in conjunction with the polyclonalantibody directed against the c4 protein revealed that c4 proteinwas associated with a subset of vascular elements (Fig. 5A). Boththe glomerular capillaries as well as peritubular capillarieswere positive for the c4 protein, and fortuitous oblique sectionsrevealed staining of the juxtaglomerular mesangial matrix (datanot shown). Interstitial tissue and renal tubules were devoidof immunoreactivity. At slightly higher magnification, overlapbetween the antigens in a subset of vessels was more readily apparent(Fig. 5B). Notably, a significant population of vessels was notstained with the antibodies directed against the c4 protein. Thesefindings were corroborated in double-labeling experiments usingantibodies directed against the circulating coagulatory proteinvon Willebrand factor as a marker for endothelia (data not shown).

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Fig. 5. Immunohistochemical localization of c4 protein to renal microvasculature. Thin sections of human kidney tissue were stained with a polyclonal antibody directed against recombinant c4 protein and monoclonal antibody A028 directed against an unspecified endothelial cell surface antigen. Fluorophore-conjugated secondary antibodies were used to visualize c4 protein (rhodamine, red) and endothelial cells (fluorescein, green). Regions of fluorophore overlap appear yellow. g, glomerular capillaries. Magnifications: A, ×630; B, ×1,000.

The observation that c4 protein was associated with a limited population of blood vessels spurred an examination of the relativeabundance of the protein in artery versus small periarterial vessels.Immunofluorescence microscopy of mesenteric artery in cross sectionrevealed a modest deposition of the c4 protein in fibrillar arraysthroughout the vascular wall of the artery. However, in sectionswhere small periarterial vessels were also present, it was evidentthat the c4 protein was markedly enriched in these vessels (Fig.6, A and B). Together these data suggested that expression ofc4 protein was most prevalent in the microvasculature. In addition,the fibrillar arrangement of the c4 protein evident in large vesselsindicated it may be a component of the extracellular matrix.

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Fig. 6. Differential expression of cablin in distinct vessel types. Thin sections of rat mesenteric artery were stained with a polyclonal antibody directed against recombinant c4 protein. Rhodamine-conjugated secondary antibody was used to visualize c4 protein in mesenteric artery and a small periarterial vessel. l, artery lumen. Magnifications: A, ×630; B, ×1,000.

c4 Protein is deposited in the basal laminae of capillaries. Immunoelectron microscopic analysis of kidney tissue was instrumentalin establishing the precise spatial relationship between microvascularendothelial cells and the c4 protein. A low-magnification micrographof a peritubular capillary in which the vessel lumen, an endothelialcell, the basal lamina, and a periendothelial cell are evidentdemonstrated an association of c4 protein with the capillary basallamina (Fig. 7A, arrows). A higher magnification view of a similarsection features the basal lamina encapsulating an endothelialcell and the process of a periendothelial cell (Fig. 7B). Goldparticles decorated c4 protein throughout the extracellular matrix,notably among fibrillar material. To facilitate visualizationof gold labeling, a detection antibody conjugated to large gold(20 nm) was used, which may account for the somewhat sparse labelingobserved. The association of c4 protein with the fibrillar matrixsurrounding capillaries prompted us to name the protein cablin(protein of the capillary basal lamina).

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Fig. 7. Immunoelectron microscopic localization of c4 protein to subendothelial basal lamina. Ultrathin sections of embedded rat kidney tissue were incubated with a polyclonal antibody directed against recombinant c4 protein and immunoreactivity was detected using gold-conjugated anti-rabbit IgG (arrows). A: low-magnification view (×6,000) of cross-sectioned capillary. B: high-magnification view (×25,000) of capillary basal lamina. en, Endothelial cell; er, erythrocyte; p, pericyte; bl, basal lamina.

Cellular expression and secretion of cablin. The close apposition between sites of cablin deposition and endothelial and periendothelialcells suggested that one or both of these cell types might beresponsible for its biosynthesis. Cellular extracts and conditionedmedia of primary cells in culture were therefore tested for cablinexpression by immunoblot analysis. Cablin was synthesized andsecreted by all cell types examined, including vein endothelialcells, microvascular endothelial cells, and aortic smooth musclecells (Fig. 8, A and B, arrow). (A slightly lower molecular weightband, seen in Fig. 8A, is thought to represent a degradation intermediate.)However, the extent of cablin secretion by different cell typeswas particularly noteworthy. Smooth muscle cells produced significantamounts of cablin (Fig. 8A), yet secretion appeared to be inefficient.Endothelial cells synthesized less cablin, but the majority ofthe protein was secreted (Fig. 8B). On the basis of these in vitrodata it is plausible that relative to other cell types endothelialcells may preferentially deposit cablin in vascular extracellularmatrices.

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Fig. 8. Cablin synthesis and secretion by cultured cells. Proteins in cellular extracts (A) or conditioned media (B) were resolved by SDS-PAGE and transferred to nitrocellulose membranes. Blots were probed with an affinity-purified antibody directed against recombinant c4 protein. Antibody binding was visualized using an HRP-conjugated secondary antibody and chemiluminescent substrate. Lane 1, aortic smooth muscle cells; lane 2, umbilical vein endothelial cells; lane 3, lung microvascular capillary endothelial cells. Equal amounts of cellular proteins were loaded (10 µg) in A, and a volume of conditioned medium corresponding to the cellular protein concentration was loaded in B. Relative migration of molecular weight standards is as indicated. Arrow, cablin.

Cablin is expressed at sites of angiogenesis. The deposition of cablin in microvascular basal laminae prompted us to examineits expression in capillaries undergoing angiogenesis. In a murinemodel of retinal neovascularization (56), hypoxia-induced stressresults in proliferation and migration of endothelial cells normallypresent only in a discrete vascular layer at the periphery ofthe retina. This response leads to the formation of angiogenictufts that invade the vitreous. Immunofluorescence microscopicanalysis of control retinas revealed that cablin colocalized withan endothelial cell marker (Fig. 9B, arrowhead) in the vascularlayer along the outer retina (Fig. 9A, asterisk). Weak cablinstaining could be detected in the cell layer immediately abovethe photoreceptor cells, but this was barely above a diffuse backgroundsignal also observed with preimmune serum (Fig. 9E). Neither endothelialcells nor cablin were detected in the layer abutting the vitreous(containing the optic nerve fibers). In contrast to control retinas,those recovered following hypoxia displayed capillary tufts consistingof 5-10 endothelial cells growing into the vitreous (Fig. 9C,arrow), and endothelial cells were seen to permeate all layersof the retina. Although cablin was apparent in the tufts themselves(Fig. 9D, arrows), the predominant immunoreactive regions wereimmediately subjacent to the tufts. This finding raises the possibilitythat recruitment of endothelial cells to sites of hypoxic injuryis correlated with the induction of cablin expression and itsassembly into a supporting extracellular matrix.

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Fig. 9. Cablin is associated with sprouting capillaries in a model of angiogenesis. Variously stained thin sections of control (A and B) or experimental angiogenic mouse retinas (D and E) are shown. A: control retina stained with hematoxylin-eosin. B: polyclonal antibody directed against recombinant c4 protein and a monoclonal antibody (A028) directed against an unspecified endothelial cell surface antigen were used to stain a control retina. Cablin staining was detected using a fluorescein-conjugated secondary antibody (green), and endothelial cells were visualized with a rhodamine-conjugated secondary antibody (red). Regions of fluorophore overlap appear yellow. C: monoclonal antibody A028 directed against an unspecified endothelial cell surface antigen was used to stain an experimental retina. Endothelium was detected using a fluorescein-conjugated secondary antibody (green) and nuclei were visualized with DAPI (blue). Because of the thickness of the section, individual nuclei are visible only in the peripheral areas of the retina. D: cablin distribution in an experimental retina was detected by staining with a polyclonal antibody directed against recombinant c4 protein followed by fluorescein-conjugated secondary antibody (green) and nuclei were visualized with DAPI (blue). E: preimmune serum was used to stain an experimental retina. Antibody binding was detected with fluorescein-conjugated secondary antibody (green). V denotes vitreous; arrowhead denotes blood vessel; arrows denote capillary tufts; 1 denotes Muller's and optic nerve fiber layer and plexiform/ganglion layer; 2 denotes bipolar, horizontal, amacrine and Muller cell layer; 3 denotes photoreceptor cell layer; asterisk denotes vascular layer (this layer is incomplete in C-E). Magnification: ×400.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

This study describes the characterization of cablin, a novel protein preferentially associated with the capillary basal lamina.The protein was synthesized and secreted by cultured microvascularendothelial cells as well as vascular smooth muscle cells, hypothesizedto be differentiated pericytes (37, 39, 48, 49). In addition,its synthesis was upregulated in tissue undergoing active neovascularization.Cablin was predominantly associated with the microvasculature,where it was specifically arrayed in the electron-lucent amorphousmaterial of capillary basal laminae. These findings offer thefirst indication that the microvascular basal lamina is biochemicallyunique. Analyses of amino acid sequence composition and predictedsecondary structure are consistent with cablin being an $alpha$ -helical,rodlike protein with domains characteristic of extracellular matrixproteins. The enrichment of cablin in vascular regions subjectto high hydrostatic pressure and shear force (including the glomerularbasement membrane and the juxtaglomerular mesangial matrix), inconjunction with a possible association with microfibrils, suggestthat cablin reinforces the architectural integrity of thetissue.

The microvasculature consists of networks of capillaries, precapillary arterioles, and postcapillary venules highly specializedfor the fundamental activities of molecular exchange and angiogenesis.Results presented here demonstrated that cablin was predominantlyassociated with the microvasculature and minimally with othervessels. Immunodetection of cablin was predicated on the relativeabundance of capillaries within the sample. The glomerular andperitubular microvasculature within the microvessel-rich kidneycortex were the exclusive sites of cablin immunoreactivity. However,examination of sections enriched in elastic and muscular vesselsrevealed that these structures were in fact immunoreactive, albeitto a lesser extent than capillaries. Here, low levels of cablinwere apparent in discrete fibrillar arrays interspersed betweenelastin fibrils. Although tissue etching has been instrumentalin revealing masked antigenic sites on extracellular matrix proteins(22), this procedure did not alter the unprecedented distributionof cablin to a subset of vascular elements (data notshown).

The vasculature represents a continuum of vessel segments that are functionally and morphologically distinct on account oftransitions in cellular phenotype. Therefore, vascular cells fromdiverse vessel populations were screened for cablin synthesis.Because of the difficulties associated with isolation and cultivationof pericytes, these cells could not be examined directly. However,on the basis of biochemical and morphological studies, severalgroups have hypothesized that pericytes differentiate into vascularsmooth muscle cells (37, 39, 48, 49). Interestingly, whenvascular smooth muscle cells were screened for cablin production,they were found to synthesize the greatest amount of protein amongthe cell types analyzed. However, microvascular endothelial cellssecreted the most cablin. Therefore, it is likely that pericytes,analogous to vascular smooth muscle cells, contribute some cablinto the capillary basal lamina, but the microvascular endothelialcells are principally responsible for its deposition. Althoughthe cellular composition of capillaries has long been recognizedas unique, these data offer the first indication that the biochemicalconstitution of capillary basal laminae is alsodistinct.

The primary amino acid sequence of cablin contains two domains implicated in cell and extracellular matrix binding: an integrin-bindingRGD motif and a putative elastin-binding sequence. The RGD tripeptidemediates the binding of extracellular matrix components to cellularintegrins (29). RGD-binding integrins found in vascular tissueinclude $alpha$ 3 $beta$ 1 and $alpha$ 5 $beta$ 1. Notably, capillary endothelial cells arethe only vascular cells that express $alpha$ 5 $beta$ 1 integrins beyond embryogenesis(41). Potential interactions between cablin and the $alpha$ 5 $beta$ 1 integrinmay stabilize cell-extracellular matrix adherence while potentiatingsignaling cascades. These possibilities are currently beingexplored.

The second identifiable domain in cablin was a 60 amino acid stretch containing 22% identity with a bacterial elastin-bindingpeptide (44). Compellingly, cablin was detected in the electron-lucentregions of the basal lamina bearing resemblance to sites of elastin-associatedmicrofibril deposition (7, 24), where it appeared in closeapposition to fibrous structures. The possible association ofcablin with microfibrils is particularly intriguing given theorganization of microfibrils into a mechanically dynamic molecularscaffold on which effector molecules areassembled.

Because of the extensive cross-linking and organization within the extracellular matrix, microfibril proteins are notoriouslydifficult to remove from tissue. Sequential tissue extractionrevealed the release of cablin in two pools (data not shown).Mild extraction conditions, including low levels of nonionic detergent,removed a portion of cablin, whereas the remainder of the proteinwas only extracted by harsh, reductive saline conditions. Cablinextracted under the mild conditions may represent a cellular orsoluble extracellular form of the protein. The pool recoveredon harsh extraction may correspond to molecules embedded in theextracellular matrix. Analogous solubilization conditions werenecessary to disrupt the association between other secreted molecules(such as latent TGF- $beta$ binding proteins and thrombospondin) andmicrofibrils (3, 21). On the basis of these morphologicaland biochemical analyses, the deposition or adsorption of cablinto microfibrils or other components of the extracellular matrixseemslikely.

Capillaries serve a unique role in both angiogenesis and metabolite exchange. Detailed morphological studies have demonstratedthat the architecture of the microvasculature is uniquely adaptedfor these functions. The structure and differentiation of thetissue is in turn dependent on the molecular composition and organizationof the extracellular matrix. It is envisaged that as a uniquecomponent of the capillary matrix, cablin could function in eithera structural or regulatory capacity. As a putative structuralcomponent of elastin-containing microfibrils, cablin may be importantin the resistance of the tissue against mechanical injury. Sucha scenario is supported by the localization of cablin to regionsof high hydrostatic pressure, the extraction properties of cablin,and the likely association of cablin with components essentialfor structural integrity. However, it is also important to considerthat angiogenic cell proliferation, differentiation, and migrationare governed by the composition of this extracellular matrix (17,26, 28, 32). Capillary sprouts are surrounded by discreteareas of extracellular matrix reorganization and synthesis (13).Therefore, the observation that cablin synthesis is induced duringneovascularization is quite compelling. Conceivably, cablin couldprovide differentiation cues or scaffolding critical for endothelialmigration during angiogenesis. Because angiogenesis is necessaryfor disease processes such as tumor progression and diabetic retinopathy,it is possible that regulation of cablin expression may influencethe angiogenic potential of tissues involved in pathological processes.Elucidation of possible structural or regulatory roles of cablin,the first unique component of the capillary basal lamina, is likelyto contribute to the understanding of processes unique to themicrovasculature.

	ACKNOWLEDGEMENTS

This study is the result of collaborative efforts between A. Wandinger-Ness and R. L. Bacallao, who contributed equally tothe supervision of the experimentsherein.

	FOOTNOTES

We thank Eugene Minner for preparing ultrathin tissue sections. Drs. Paul McGuire and Nancy Kanagy graciously provided sectionsof retinas and mesenteric artery, respectively. Dr. Richard Larsonand David Brown supplied valuable cell cultures. We also thankDrs. Nancy Kanagy and Richard Larson for critically reading thepaper.

This work was supported by the National Institute of Diabetes and Digestive and Kidney Diseases Grants R01 DK-50141 (to A.Wandinger-Ness) and R29 DK-46883 to (R. L. Bacallao). A. Wandinger-Nessis the recipient of start-up funds provided by a Howard HughesMedical Institute Research Resources for Medical Schools Award(76296-550501). A. J. Charron was partially supported by a NationalInstitutes of Health Predoctoral Training Grant T32 GM-08061.

The costs of publication of this article were defrayed in part by the payment of page charges. The article must thereforebe hereby marked "advertisement" in accordance with 18 U.S.C.§1734 solely to indicate thisfact.

Address for reprint requests and other correspondence: A. Wandinger-Ness, Dept. of Pathology, CRF 225, 2325 Camino de Salud, Univ. of New Mexico Health Sciences Center, Albuquerque, NM 87131 (E-mail: wness{at}unm.edu).

Received 12 April 1999; accepted in final form 14 June 1999.

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