Isolation of rat fibrillin-1 cDNA and its relevance in metanephric development

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Isolation of rat fibrillin-1 cDNA and its relevance in metanephric development

Yashpal S. Kanwar, Kosuke Ota, Qiwei Yang, Anil Kumar, Jun Wada, Naoki Kashihara, and Darryl R. Peterson

Department of Pathology, Northwestern University Medical School, Chicago, Illinois 60611

ABSTRACT

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

The role of fibrillin-1 in metanephrogenesis was investigated. Fibrillin-1 cDNA was isolated from the rat kidney cDNA libraryand sequenced, and its spatiotemporal expression was studied.It had ~88% homology with human fibrillin-1 and had Ca²⁺ binding epidermal growth factor-like domains, transforming growthfactor- $beta$ binding protein motifs, and an RGD binding site. Northernblot analysis revealed an ~10-kb transcript, and fibrillin-1 expressionwas developmentally regulated. In situ hybridization and immunofluorescencestudies indicated that at day 15 of gestation, fibrillin-1 isexpressed in the metanephric mesenchyme. At day 18, its expressionwas confined to nascent blood vessels and glomeruli, and it increasedin the newborn and neonatal kidneys. Immunoprecipitation revealedan ~300-kDa band by SDS-PAGE. Treatment with fibrillin-1 antisenseoligodeoxynucleotide induced marked dysmorphogenesis of the embryonicmetanephroi. Concomitantly, the fibrillin-1 mRNA, antibody reactivityin the metanephroi, and fibrillin-1-specific radioincorporationwere reduced. These data indicate that, like $alpha$ _v $beta$ ₃ integrin, aknown morphogen and a putative receptor of fibrillin-1, the fibrillin-1modulates events related to early organogenesis and possibly alsothe vascularization of the ratkidney.

fibrillin; complementary deoxyribonucleic acid cloning; extracellular matrix

	INTRODUCTION

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AMONG THE COMPONENTS of the extracellular matrix (ECM), there are various nonstriated fibrils, known as microfibrils, whichare classified by the size of their diameters (24, 27, 29,33). Fibrillin-1 and -2 seem to be the major structural componentsof the beaded 10- to 14-nm microfibrils that are widely distributedin elastic and nonelastic tissues (9, 10, 18). In elastictissues like the aorta, fibrillin-1-associated microfibrils arethought to play a role in the formation of elastic fibers, thusallowing them to generate an elastic recoil (4, 24). Conversely,in nonelastic tissues they may anchor epithelial cells to theinterstitial matrix and therefore participate in various biologicalprocesses, e.g., wound healing and embryonic development (42,43). The structure of human fibrillin-1 and -2 has been described,and mutations in the genes have been found in Marfan syndrome,which is associated with connective tissue abnormalities of theeye, skeletal system, and cardiovascular system (6, 15, 20,23, 26, 39). The cDNA sequence of fibrillin-1 in human andmouse is highly conserved (6, 23, 42). Analysis of thelatter indicates that it is a modular protein, consisting of 48epidermal growth factor (EGF)-like domains, 7 domains homologousto transforming growth factor- $beta$ 1 (TGF- $beta$ 1) binding protein (8-cysteinemotifs), a fibrillin motif, a fibrillin-like module, a 57 aminoacid proline-rich domain, a single RGD coding sequence, and uniqueamino and carboxy termini (23, 27, 29, 34, 42). Most(43/48) of the EGF-like domains have Ca²⁺-binding (cb) sites (5, 12, 28). Such cbEGF-like domainsare believed to be involved in protein:protein interactions andhave been found in other ECM proteins like fibulin-1 and -2, nidogen,and versican (12, 13, 28, 30, 31, 36).

Conceivably, the structural and biochemical characteristics of fibrillin-1, i.e., RGD sequence and cbEGF-like domains, asseen in some of the ECM proteins, may be relevant to the variousbiological processes prevalent during embryonic development. Forinstance, the RGD sequence mediating fibroblast attachment tofibrillin-1 is sensitive to inhibition by antibodies to the $alpha$ _v $beta$ ₃-integrinreceptor (34), which has been shown to regulate metanephricdevelopment. Second, nidogen that contains cbEGF-like domainsinteracts with another major ECM protein, laminin, and both seemto regulate tubulogenesis during renal development (7). Third,cbEGF-like domains are present in neurogenic loci Notch and Delta,the two EGF-homologous genes in Drosophila (8, 28). Theirexpression in nonadhesive Drosophila Schneider's 2 (S2) cellsinduces aggregation, suggesting their role in protein:proteinand cell:cell interactions (8), with the latter necessary fororganogenesis during embryonic development. In view of the aboveconsiderations, studies were initiated to delineate the role offibrillin-1, a protein with multiple cbEGF-like domains (27,29), in rat development by utilizing the rat metanephric culturesystem.

	MATERIALS AND METHODS

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Animals. Sprague-Dawley rats (Harlan Sprague Dawley, Indianapolis, IN) were used for paired male-female mating, and the appearanceof the vaginal plug was designated as day 0 of fetal gestation.Kidneys from embryonic rats were harvested aseptically at days15 (E15) and 18 (E18) of gestation, and in addition, kidneys wereobtained from the newborn and 1-, 2-, and 3-wk-oldrats.

Construction of newborn rat kidney cDNA library. Total RNA from ~100 newborn rat kidneys was isolated by the guanidinium isothiocyanate-CsClcentrifugation method (2). Poly(A)⁺ RNA was selected by oligo(dT)-cellulose chromatography. First-strandcDNA was synthesized by using Moloney murine leukemia virus reversetranscriptase (MMLV-RT, RNase H) and oligo(dT)₂₅d(G/C/A) as a primer (Clontech, Palo Alto, CA).Double-stranded cDNA was prepared by the RNase H-DNA polymeraseI method for second strand synthesis (17). After ligation ofEcoR I-Not I-Sal I adapters and polynucleotide kinase phosphorylation,the double-stranded cDNA was size-fractionated, and small DNAfragments, i.e., <400 bp, were removed by a Chromaspin-1000 column(Clontech). The cDNA was ligated into an EcoR I-digested and dephosphorylated $lambda$ -ZAP II vector and packaged using Gigapack II Gold PackagingExtract (Stratagene, La Jolla, CA). The packaged ligation productwas incubated with E. coli XL1-Blue MRF' cells for plating andtitration of recombinant phage plaques (17).

Screening of rat newborn rat cDNA library and isolation and nucleotide sequence analyses of fibrillin-1 cDNA clones. A mousefibrillin-1 cDNA, previously isolated in our laboratory (GenBankaccession no. U22493), was used for screening the rat newborncDNA library. About 2 × 10⁶ recombinants were screened with [ $alpha$ -³²P]dCTP-labeled mouse fibrillin cDNA. Nitrocellulose filter lifts(Schleicher and Schuell, Keene, NH) were made, then prehybridizedand hybridized with the radiolabeled screening probe as previouslydescribed (40). Several clones were isolated, then purifiedby dilutional secondary and tertiary screenings. The clones containingcDNA inserts, which strongly hybridized with the screening probe,were processed for further subcloning. Eleven overlapping cloneswere isolated and subcloned into pBluescript II KS(+) phagemidusing XL1-Blue MRF' cells (Stratagene). For rescuing of single-strandedDNA, the transfected cells were grown in the presence of VCSM13helper phage. The supernatants of the cultures were saved, andsingle-stranded DNA was isolated by polyethylene glycol precipitation.After the sense or antisense orientation of various subcloneswas determined, nucleotide sequencing was performed by the dideoxychain termination method (35), followed by hydropathic (19)and sequence homology analyses (22) using the Wisconsin PackageVersion 9.1-UNIX (Madison,WI).

Gene expression studies by Northern blot analysis and in situ hybridization. Total RNA from embryonic kidneys at various stagesof gestation and from kidneys of 1- and 3-wk-old rats was extractedby the guanidinium isothiocyanate-CsCl centrifugation method (2).Equal amounts of RNA, extracted from rat kidneys at various stagesof gestation and the neonatal period, were glyoxalated and subjectedto 1% agarose gel electrophoresis in 10 mM sodium phosphate buffer,pH 7.0. A Northern blot was prepared by transferring the RNA toa nylon filter membrane (Amersham, Arlington Heights, IL) andhybridizing with [ $alpha$ -³²P]dCTP-labeled rat fibrillin-1 cDNA. The filter was washed underhigh-stringency conditions with 0.1× SSC and 0.1% SDS at 60°C,and autoradiograms were prepared. After stripping, the same blotwas also hybridized with a $beta$ -actin probe (GenBank accession no.M62174; American Type Culture Collection, Rockville, MD), andthe autoradiogram was prepared as describedabove.

For in situ hybridization studies, first a PCR product of 771 bp was prepared by using the primers, derived from rat fibrillin-1cDNA. The respective sense and antisense primers were as follows:5'-CATCCGCACTGGAGCTTGTC-3' and 5'-CACTCATCAACGTCGATGC-3'. Thisfibrillin-1 cDNA PCR product was ligated into pBluescript KS(+)and used as a template for generating sense and antisense riboprobesby using the Riboprobe In Vitro Transcription System (Promega,Madison, WI). The riboprobes were synthesized by incorporating[ $alpha$ -³³P]UTP (Amersham), using T3 and T7 RNA polymerases and the linearizedPCR product of rat fibrillin-1 cDNA. The radiolabeled riboprobeswere subjected to limited alkaline hydrolysis to yield polynucleotidefragments of 100-150 bp size, which were then used for in situhybridization with the tissue sections (17, 40).

Embryonic (E15 and E18), newborn, and 1- and 3-wk-old rat kidneys were immersed in 4% paraformaldehyde in PBS, pH 7.0, for3 h at 4°C. The tissue specimens were then dehydrated, and embeddedin paraffin. Tissue sections, 3 µm thick, were prepared and mountedon glass slides coated with Vectabond (Vector Laboratories, Burlingame,CA). The sections were deparaffinized, hydrated, treated with0.2 N HCl, deproteinated by proteinase K treatment, and acetylatedwith 0.1 M triethanolamine and 0.25% acetic anhydride. After thesections were washed with 2× SSC, they were prehybridized withhybridization solution (50% formamide, 10% dextran sulfate, Denhardt'ssolution in 10 mM Tris · HCl, pH 8.0) at 50°C for 3 h, then hybridizedwith [ $alpha$ -³³P]UTP-labeled fibrillin riboprobes at 50°C for 15 h. After hybridization,the tissue sections were washed with 50% formamide in 2× SSC,treated with RNase A, and rewashed with 0.1× SSC at 50°C. Thesections were then dehydrated, air-dried, and coated with NTB2photographic emulsion (Eastman Kodak, New Haven, CT), and tissueautoradiograms were prepared after 1-2 wk ofexposure.

Generation of anti-fibrillin-1 antibody and its characterization. To raise a polyclonal antibody to fibrillin-1, a syntheticpeptide was prepared with the following amino acid sequence: RPPPEYPYPSPSREPPK.This stretch of amino acids is boldly underscored in Fig. 1A.An additional lysine residue was added to the NH₂ terminus ofthe peptide for its conjugation with keyhole limpet hemocyanin.One milligram of conjugated peptide was mixed with complete Freund'sadjuvant and used for immunizing rabbits. Booster injections ofthe antigen were given every 3 wk, and rabbit antisera were collected.An IgG fraction was prepared from the antisera by ammonium sulfateprecipitation, as previously described (41). The purified IgGfraction was dialyzed against PBS, lyophilized, and stored at $-$ 70°C.

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Fig. 1. Nucleotide and deduced amino acid sequence of full-length rat fibrillin-1 cDNA. Shaded box (top left in A): sequence antisense oligodeoxynucleotide (ODN) used in organ culture experiment. Open box (bottom right in A): location of the RGD sequence. Bold underscore (middle left of A): amino acid sequence of the synthetic peptide used for the generation of the antibody. Underscore (right in B): sense and antisense primers used for the competitive RT-PCR analyses.

The specificity of the antibody was established by ELISA, the procedural details of which have been described previously (41).Briefly, wells of an EIA/RIA plate were coated with 5 µg of syntheticpeptide, followed by washing with methanol and blocking with bovineserum albumin. After two washes with PBS, 0.5 µg of the antibody(IgG fraction) was added to the first well, and log dilutionsof the antibody were made in successive wells. Incubation wascarried out for 1 h, and the wells were rewashed with PBS containing0.05% Tween-20. Horseradish peroxidase-conjugated goat anti-rabbitIgG (Cappel; Organon Teknika, Durham, NC) diluted 1:1,000 wasadded and incubated for 30 min. After three rewashings, a colorimetricreaction was carried out with tetramethylbenzidine solution (Bio-RadLaboratories, Hercules, CA), and the reaction was stopped withthe addition of 0.3 M H₂SO₄. Finally, readings at OD₄₉₀ were madeand plotted against the log dilutions of the antibody. For a competitiveinhibition ELISA assay, 250 µg of the synthetic peptide were addedin the first well of the peptide-coated EIA/RIA plate along with0.5 µg of the antibody. Log dilutions of the synthetic peptidewere made in successive wells while the concentration of the primaryantibody was kept constant. Conditions for incubation with secondaryantibody and colorimetric reactions were the same as describedabove. Readings at OD₄₉₀ were made and plotted against the logdilutions of theantigen.

The specificity of the antibody was also determined by immunoprecipitation methods (41). About 100 E15 metanephroi wereharvested and maintained in an organ culture system, as detailedpreviously (21). Briefly, harvested metanephric explants wereplaced on a 0.8-µm pore size filter and floated onto a serum-freemedium. The latter was made up of equal volumes of DME and Ham'snutrient mixture F-12, penicillin (100 µg/ml), streptomycin (100µg/ml), and transferrin (50 µg/ml) (Sigma Chemical, St. Louis,MO). The explants were cultured in a CO₂ incubator for 4 daysand then radiolabeled with [³⁵S]methionine (0.25 mCi/ml) for 16 h prior to the termination ofthe culture. They were lysed in an extraction buffer [6 M guanidine-HCl,100 mM Tris · HCl, pH 7.5, 0.02% NaN₃, 10 mM $epsilon$ -amino-n-caproicacid, 5 mM N-ethylmaleimide, and 1 mM phenylmethylsulfonyl fluoride(PMSF)] by shaking vigorously for 6 h at 4°C. The extract wascentrifuged at 10,000 g for 30 min at 4°C. Ten volumes of ethanolwere added to the supernatant to precipitate the extracted proteinat $-$ 20°C for 15 h. The precipitate was centrifuged at 10,000 gfor 30 min at 4°C, and the pellet was resuspended in the immunoprecipitationbuffer and saved. The immunoprecipitation buffer consisted of0.1% SDS, 1% Triton X-100, 50 mM Tris · HCl, pH 7.5, 50 mM NaCl,0.02% NaN₃, 0.25 mM dithiothreitol, 10 mM benzamidine-HCl, 10mM $epsilon$ -amino-n-caproic acid, 5 mM N-ethylmaleimide, and 1 mM PMSF.Immunoprecipitation was performed by adding 5 µl of polyclonalanti-fibrillin-1 antibody to 0.5 ml (5 × 10⁶ dpm) of the sample. The mixture was gently swirled in an orbitalshaker for 15 h at 4°C. After addition of 80 µl of protein-A-Sepharose4B (Pharmacia LKB Biotechnology, Piscataway, NJ), the antigen-antibodymixture was further incubated for 1 h at 4°C. The antigen-antibodycomplex was washed three times with the buffer, then dissolvedin a sample buffer (4% SDS, 150 mM Tris · HCl, pH 6.8, 20% glycerol,0.1% bromophenol blue, and 10% $beta$ -mercaptoethanol), boiled for5 min, and subjected to 5% SDS-PAGE analysis. The gels were thenfixed in 10% acetic acid and 10% methanol, treated with 1 M salicylicacid, and vacuum dried, and autoradiograms were prepared. Twocontrol immunoprecipitation experiments were also performed. Inthe first, polyclonal anti-fibrillin-1 antibody, previously absorbedwith the synthetic peptide, was used for immunoprecipitation;in the second, preimmune rabbit serum was used as a control. Inboth the controls, double the amount of immunoprecipitated radioactivitywas used in SDS-PAGE analyses to ensure the specificity of theantibody.

Fibrillin-1 expression by tissue immunofluorescence. Kidneys of E15 and E18 embryos and of newborn and 1-, 2-, and 3-wk-oldrats were snap frozen in chilled isopentane and embedded in OCTcompound (Miles Laboratories, Elkhart, IN). Cryostat sections,4 µm thick, were prepared and air-dried. Sections were washedwith 0.01 M PBS, pH 7.4, and incubated with polyclonal anti-fibrillin-1antibody, with 1:100 dilution, for 30 min in a humidified chamberat 37°C. After washing with PBS, sections were reincubated withgoat anti-rabbit IgG antibody and conjugated with fluoresceinisothiocyanate for 30 min. The sections were rewashed with PBS,covered with a drop of buffered glycerol, coverslip mounted, andexamined with an ultraviolet microscope equipped with epi-illumination.

Antisense experiment. The antisense experiments were performed to determine the role of fibrillin-1 in the organogenesis ofembryonic kidneys. A sense-, two nonsense-, and antisense-phosphorothioatedoligodeoxynucleotides (ODN) were synthesized by an automated solid-phasesynthesizer (Biotech facility, Northwestern University) and purifiedby high-performance liquid chromatography. The 35-mer sense/antisenseODN sequence was selected from the 5' end of the cloned rat fibrillin-1,and it is as follows: 5'-GCCAGCGCGACCTCCAGCAGCCCTCCTCGCCGCAT-3'(Fig. 1). Its specificity for the target nucleotide sequenceswas established by S₁ nuclease protection assays as describedpreviously (see Fig. 5D and see RESULTS). Two nonsense 31-merphosphorothioated ODNs were also prepared for these experiments,and their sequences were as follows: 5'-TAATGATAGTAATGATAGTAATGATAGTAAT-3'and 5'-GATCGATCGATCGATCGATCGATCGATCGAT-3'. Both the ODNs (antisenseand nonsense) did not exhibit any significant homology with othermammalian nucleotide sequences available in the GenBankdatabase.

About 600 rat embryonic kidneys at day 15 (E15) of gestation were harvested and maintained in culture for 4 days. The ODNswere added to the culture media daily at a concentration of 0.5µM. At this concentration, the ODNs retain the translational blockadespecificity with no discernible cytotoxic effects (1, 17,40). The metanephric explants (200 kidneys per variable, i.e.,sense, antisense, and nonsense) were processed for light microscopy,quantitative RT-PCR analyses, and immunofluorescence and immunoprecipitationstudies. For light microscopy, the sections from the midplaneof the embryonic kidneys with a maximum number of ureteric buditerations, including both the poles and the hilus, were evaluatedas described previously (17, 40).

Quantitative RT-PCR analyses of fibrillin-1 mRNA of antisense ODN-treated metanephroi. To assess the effect of antisense ODNson mRNA expression, competitive RT-PCR analyses were carried outas described previously (17, 40). Total RNAs were isolatedfrom 50 explants per variable by an acid guanidinium isothiocyanate-phenol-chloroformextraction method (3). Extracted RNAs were treated with RNase-freeDNase (Boehringer Mannheim, Indianapolis, IN), followed by anethanol precipitation. About 25 µg of total RNAs, from each variable,were subjected to first-strand cDNA synthesis using MMLV-RT andoligo(dT) as a primer. The cDNAs from different variables weresuspended in 25 µl of deionized autoclaved water and kept at $-$ 70°Cuntil furtheruse.

For the analyses of fibrillin-1 mRNA, the respective sense and antisense primers were 5'-GATCATATCACTGCATCTG-3' and 5'-GAGCAACCATAACTGCAGG-3'.Their locations in the rat fibrillin-1 cDNA are indicated in Fig.1B as underscored nucleotide sequences. For $beta$ -actin, the respectivesense ( $beta$ -SE) and antisense ( $beta$ -AS) primers were 5'-GACGACCATGGAGAAGATCTGG-3'and 5'-GAGGATGCGGCAGTGCGGAT-3' (38). Using these primers, weexpected the PCR product sizes to be 723 bp for rat fibrillin-1and 461 bp for $beta$ -actin, and their nucleotide sequences were confirmedby the dideoxy chain termination method (35). The 723-bp PCRproduct was then used for the preparation of a competitive DNAtemplate for fibrillin-1. A Hinc II site was introduced by usinga nested primer with the sequence 5'-GGGTAACCACCGCTGCCAACTGG-3',and the resulting PCR product was ligated into pCR II vector (Invitrogen,San Diego, CA). The plasmid with this cDNA insert was digestedwith Hinc II (Boehringer Mannheim) to delete the 229-bp fibrillin-1DNA fragment flanked by Hinc II sites. The digested plasmid waspurified by agarose gel electrophoresis and subjected to self-ligationwith DNA ligase (Boehringer Mannheim). The plasmid, containingthe truncated 494-bp fibrillin-1 insert, was linearized with appropriaterestriction enzyme digestion and used as a competitive DNA templatefor fibrillin-1 mRNA analyses by RT-PCR. The construction of acompetitive 224-bp DNA template for $beta$ -actin has been describedin our previous publications (17, 40; GenBank accession no. U17140).

For quantitative RT-PCR analyses, a fixed amount of cDNAs (1 µl) from antisense and nonsense ODN-treated metanephroi and seriallogarithmic dilutions of the competitive template DNA (500 ng/µl)of fibrillin-1 were coamplified (11). The reaction mixture included5 µl of 10× PCR buffer, 250 µM of each dNTPs, 1 µM of sense andantisense primers, and 1 U Taq polymerase (Perkin-Elmer, Norwalk,CT) in a total volume of 50 µl. The amplification reaction wascarried out for a total of 30 cycles in a DNA Thermal Cycler (Perkin-Elmer),each cycle consisting of denaturation at 94°C for 1 min, annealingat 60°C for 1 min, and extension at 72°C for 1 min. The PCR productsof wild-type and mutant fibrillin-1 (competitive truncated DNAtemplate) were analyzed by 2% agarose gel electrophoresis andphotographed using an instant positive/negative film (Polaroid,Cambridge, MA). The negatives were analyzed by a scanning densitometer(Hoefer Scientific Instruments, San Francisco, CA), and the relativearea underneath the tracings was computed. Similarly, the wild-typeand mutant $beta$ -actin were analyzed. The ratios between the densitometricreadings of wild-type and mutant PCR-DNA products were plottedusing a logarithmic scale on the ordinate (y-axis) against thelogarithmic dilutions of the competitive truncated template DNAon the abscissa (x-axis).

Fibrillin-1 expression in antisense ODN-treated rat metanephric explants. To assess the translational blockade of fibrillin-1,immunoprecipitation and immunofluorescence studies were performedon metanephroi treated with various ODNs, i.e., antisense, sense,and nonsense, for 48 h. For immunoprecipitation experiments, [³⁵S]methionine-labeled metanephroi were processed for SDS-PAGE analysesas described above. The controls included the untreated metanephroiand those treated with sense and nonsense ODNs. To ensure theeffect of antisense ODN on the translational blockade of rat fibrillin-1,double the amount of immunoprecipitated radioactivity was usedfor SDS-PAGE analyses. Finally, the tissue expression of fibrillin-1in antisense and sense or nonsense ODN was assessed by immunofluorescencemicroscopy as describedabove.

	RESULTS

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Characterization of newborn rat fibrillin-1 cDNA clones. Eleven clones were isolated from a newborn rat kidney library thathad overlapping sequences and common restriction sites, indicatingthat they contained identical cDNA. Clone 4 had the initiationcodon, and clone 7 had the termination codon. By combining thenucleotide stretches with shared sequences of various clones,an open-reading frame consisting of 8,616 nucleotides was obtained,which had a deduced translated product of 2,872 amino acids (Fig.1). Rat fibrillin-1 had ~88% and ~96% sequence homology with humanfibrillin-1 (26) at the nucleotide and amino acid levels, respectively.The sequence homology with the mouse fibrillin-1 gene was ~94%and ~98% at the nucleotide and amino acid levels, respectively(42). The amino acid sequence had similar structural domainsto that of the human and mouse fibrillin-1 (26, 42). Its domainstructure was characterized by a proline-rich domain stretchingfrom amino acids 391 to 450, which contained 41.6% proline residues.This domain was flanked by 8 and 49 cysteine-rich repeats upstreamand downstream, respectively. The majority of the cysteine-richrepeats had calcium binding consensus sequences, derived fromcbEGF repeats of several different proteins (36). The latter,i.e., Ca²⁺-binding EGF-like domains, are thought to be involved in mediatingprotein:protein interactions (28). The downstream cysteine-richrepeats domain also contained six TGF binding protein repeatsand a fibrillin motif. Another TGF binding protein-like repeatand a fibrillin-like module were present in the upstream cysteine-richrepeatsdomain.

Expression of fibrillin-1 mRNA. Northern blot analyses revealed a single mRNA transcript of ~10 kb size in kidneys harvestedfrom E15 and E18 embryos and newborn and 1- and 3-wk-old rats(Fig. 2, top). The mRNA expression for fibrillin-1 at E15 of gestationwas detectable when ~50 µg of total RNA, isolated from ~80 explants,was used. After a mild decrease at E18, the fibrillin-1 mRNA expressionsteadily increased during various developmental stages, and wasmaximal in kidneys of 3-wk-old rats. Thereafter, the mRNA expressionleveled off, suggesting that fibrillin-1 is developmentally regulated.The mRNA expression of $beta$ -actin in the rat kidneys was constantthroughout the embryonic, neonatal, and postnatal periods (Fig.2, bottom). Since the fibrillin-1 gene seemed to be developmentallyregulated, in situ hybridization studies were performed to assessits spatial distribution in embryonic and neonatal kidneys (Fig.3). At E15, the mRNA expression was found to be restricted tothe rat metanephric loose mesenchyme, and no message was foundin the ureteric bud epithelia or in the nascent nephron (Fig.3, A and D). Interestingly, the fibrillin-1 message was observedaround the ureteric bud branches and developing nephrons (Fig.3D). Also, like some of the other ECM proteins, i.e., proteoglycans,the message was slightly concentrated on the tips of the uretericbud branches (arrowhead in Fig. 3D). At E18, the fibrillin-1 expressionwas similar to that observed at E15. In newborn kidneys, the messagewas mainly found on the mature glomeruli, and it was somewhatconcentrated in their mesangial regions (Fig. 3, B and E). Occasionally,the fibrillin-1 message was also detectable in the small intrarenalblood vessels, e.g., afferent arterioles (arrow in Fig. 3E). Amild degree of expression was observed in the interstitium insome of the tissue autoradiograms of the newborn kidneys. At 3wk, besides glomeruli, a high degree of expression was observedin large intrarenal as well as extrarenal blood vessels (Fig.3, C and F). The expression was notably high in hilar blood vesselslined with elastic lamina (Fig. 3F), whereas no expression wasobserved in tributaries of the renal vein. The expression in therenal interstitium decreased to a minimal degree in kidneys of3-wk-old rats. In kidneys of 1- and 2-wk-old rats an increasingfibrillin-1 mRNA expression in the blood vessels was observed.The adjacent kidney sections hybridized with sense riboprobesyielded a mild background signal (Fig. 3, G-I).

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Fig. 2. Northern blot analyses of rat fibrillin-1 mRNA expressed in various developmental stages of the rat kidney. A major transcript of ~10 kb for rat fibrillin-1 is observed at day 15 (E15) of the gestation. After a mild decrease at day 18 (E18), its expression increases progressively during the gestational and postnatal periods in developing kidneys. Expression of $beta$ -actin remains constant. Lanes 15d and 18d: renal mRNA from 15- and 18-day-old fetuses. Lanes NB, 1W, and 3W: newborn and 1- and 3-wk-old rat renal mRNAs.

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Fig. 3. Dark-field light microscopic autoradiogram of renal tissue sections in situ hybridized with specific fibrillin-1 riboprobe. Kidney sections from E15 (A, D, and G), newborn (B, E, and H), and 3-wk-old rats (C, F, and I) were hybridized with [ $alpha$ -³⁵S]dUTP antisense (A-F) or sense (G-I) riboprobes. At E15 (A and D), fibrillin-1 mRNA is expressed in the metanephric mesenchyme (m) surrounding the nascent nephron (n) and ureteric bud branches (u). At places the message was seen concentrated at the tips of ureteric bud branches (arrowhead in D). In newborn rat kidney (B and E), fibrillin-1 mRNA is expressed in glomeruli (g) and occasionally in afferent arterioles (arrow in E). In the 3-wk-old rat kidney, mRNA is heavily expressed in the intrarenal (C) and extrarenal (F) arterial blood vessels (v), in addition to the glomeruli. A background signal is observed in kidney tissues hybridized with sense probe (G-I). Arrows in G mark the boundary of the embryonic metanephros, and dots in I outline a venous channel.

Characterization of anti-fibrillin-1 antibody. A polyclonal anti-fibrillin-1 antibody was raised using a synthetic peptide,the sequence of which is boldly underscored in Fig. 1A. This sequenceis identical in both the mouse and rat species. The specificityof the antibody was characterized by ELISA and immunoprecipitationmethods. In the ELISA assay, a fixed amount of antigen, i.e.,synthetic peptide, and serial log dilutions of the antibody wereused. With increasing dilutions of the antibody, a proportionaldecrease in OD₄₉₀ readings was observed (solid line in Fig. 4A).To confirm the antibody specificity, an inhibition ELISA assaywas performed in which synthetic peptide was used as a competitiveantigen. With increasing dilutions of the competitive antigen,a proportional increase in OD₄₉₀ readings was observed (brokenline in Fig. 4A), indicating the specificity of the anti-fibrillinantibody. No change in the optical density readings was observedwhen synthetic peptide with sequences derived from fibrillin-2was used. For immunoprecipitation, the embryonic explants wereradiolabeled with [³⁵S]methionine, and the tissue extract was prepared. The extractwas immunoprecipitated with anti-fibrillin-1 antibody preparedin two different rabbits. The immunoprecipitates were then subjectedto 5% SDS-PAGE analyses. A single ~300-kDa band, similar to thesize of human fibrillin-1, was observed for antibodies preparedin both the rabbits (Fig. 4B, lanes 2 and 3). This indicated thatthe antibody bound specifically to the putative fibrillin-1 polypeptide.No autoradiographic band was observed when the immunoprecipitationwas performed with preimmune serum (Fig. 4B, lane 1), or whenthe antibody was preabsorbed with the synthetic peptide (Fig.4B, lane 4). In these latter two controls, double the amount ofradioactivity was loaded in lanes 1 and 4 to ensure that therewas no detectable nonspecific binding to the fibrillin-1 polypeptide.

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Fig. 4. A: ELISA and competitive-inhibition ELISA profiles of fibrillin-1 antibody and the synthetic peptide, RPPPEYPYPSPSREPPK. A decrease in OD₄₉₀ optical density readings is observed with increasing log dilutions of the anti-fibrillin-1 antibody (solid line), whereas an increase in OD₄₉₀ readings is observed with increasing log dilutions of the competitive antigen, i.e., synthetic peptide (dotted line). No change in optical density readings was observed when synthetic peptide with sequences derived from fibrillin-2 was used. B: SDS-PAGE autoradiogram of de novo synthesized and immunoprecipitated fibrillin-1. Metanephroi were radiolabeled with [³⁵S]methionine, and extracts were immunoprecipitated with anti-fibrillin-1 antibody. De novo synthesized fibrillin-1 is visualized as a band of ~300 kDa M_r as indicated by the large arrow for lanes 2 and 3. No band is seen either in preimmune serum (lane 1) or in antiserum preabsorbed with the synthetic peptide (lane 4). Small arrow indicates the point of application. C-H: immunofluorescence micrographs representing kidney tissues harvested from E15 (C) and E18 fetuses (D), newborn (E), and 1- (F), 2- (G), and 3-wk-old (H) rats. Immunofluorescence findings confirm the results obtained in gene expression studies. At E15 of gestation (C), immunoreactivity is confined to mesenchyme (*) and tissues surrounding the ureteric bud branches (u) and nascent nephrons (n). At E18 (D), reactivity is reduced, and it is confined to residual mesenchyme or interstitium (*) and around the blood vessels (v) and nephrons (arrows). In newborn kidney (E), immunoreactivity is mainly confined to glomerular mesangium (g) and blood vessels (v), while mild reactivity is seen in interstitium surrounding the tubules (arrows). Immunoreactivity in glomeruli (g) and blood vessels (v) is progressively accentuated in kidneys of 1- (F), 2- (G), and 3-wk-old (H) rats.

Immunofluorescence studies. Tissue expression was assessed by using the polyclonal anti-fibrillin-1 antibody in embryonicand neonatal rat kidneys. At E15 of gestation, the immunoreactivityof fibrillin-1 was observed in the loose metanephric mesenchyme.The fibrillin-1 was expressed as wrinkled filamentous structures,which seemed to surround the developing nephrons and the uretericbud iterations (Fig. 4C). This expression was comparable to thespatiotemporal mRNA expression of fibrillin-1 (Fig. 3, A and D).No immunoreactivity was observed in the epithelial componentsof the embryonic metanephros. At E18, immunoreactivity was notablyreduced, and it was confined to the interstitium and loose mesenchymethat had not yet been populated with developing nephrons (Fig.4D). Interestingly, mild immunoreactivity with newly formed smallblood vessels was also noted. At day 22 (newborn), immunoreactivitywas seen in mature glomeruli and blood vessels (Fig. 4E). Thevessels with elastic lamina exhibited intense reactivity. Mildimmunoreactivity of the antibody could be observed in the interstitiumas well. At 1, 2, and 3 wk, the immunoreactivity in the bloodvessels and in the glomeruli was further accentuated, whereasthat in the interstitium was considerably diminished (Fig. 4,F-H). The glomerular mesangium also exhibited a steady increasein the expression of fibrillin-1. The findings of the proteinexpression studies are comparable to the results obtained by insitu experiments. Both these studies indicate that fibrillin-1has a spatiotemporal expression in the mammalian embryonic metanephrosand thus may play a role in metanephricdevelopment.

Role of fibrillin-1 in rat renal development (antisense experiments). To study the role of fibrillin-1 in rat metanephrogenesis,gene disruption experiments, employing an antisense ODN strategy,were performed. Fibrillin-1-specific antisense ODN was used forthese experiments. Its nucleotide sequence was derived from the5' end of the fibrillin-1 gene (shaded box in Fig. 1). The specificityof fibrillin-1 antisense ODN was established by S₁ nuclease protectionassay, as detailed in previous publications (17, 40). A singleband of radioactivity, corresponding to the size of the ODN, i.e.,35-mer, was observed at 35°C, 40°C, 45°C, and 50°C hybridizationtemperatures (Fig. 5D; lanes 1, 3, 5, and 7, respectively). Noband of radioactivity was seen in the control (nonsense ODN) samples(Fig. 5D; lanes 2, 4, 6, and 8). The morphological changes inducedby the antisense ODN exposure to the embryonic metanephroi aredepicted in Fig. 5C. An overall moderate reduction in the sizeof the metanephric explant was observed compared with the untreatedcontrol (Fig. 5A) or samples treated with sense/nonsense ODN (Fig.5B). A notable decrease in iteration of the ureteric bud brancheswas seen. Also, the ureteric bud branches were disorganized, andthere was a loss of acuteness of their tips (arrow heads in Fig.5C). The metanephric mesenchyme was loosely organized and expanded,and mesenchymal cells appeared to be shrunken or atrophic. Withthe disorganization of the ureteric bud branches and atrophy ofthe mesenchymal cells, the population of glomerular and tubularelements remarkably decreased. A mild reduction in the size ofthe metanephric explant treated with nonsense ODN was observed;however, no abnormalities in the ureteric bud iterations or decreasein the population of nascent nephrons was noted. No discerniblecytotoxic effects, in the form of necrosis, were apparent in explantstreated either with antisense or sense/nonsense ODNs.

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Fig. 5. A-C: light photomicrographs of untreated (A), sense/nonsense ODN-treated (B), and antisense ODN-treated (C) rat metanephric explants. Antisense ODN-treated explant shows dysmorphogenesis of the ureteric bud branches (u) and a reduced population of glomerular and tubular elements in the loose uninduced metanephric mesenchyme. In addition, there is a loss of acuteness of the tips of ureteric bud branches (arrowheads in C), the site where epithelial:mesenchymal interactions take place. D: autoradiogram of S₁ nuclease digests of antisense ODN:RNA hybrids. Lanes 1, 3, 5, and 7 represent 5 µg of metanephric kidney mRNA hybridized with antisense ODN at 35°C, 40°C, 45°C, and 50°C, respectively, followed by S₁ nuclease digestion. A single band of radioactivity, corresponding to the size of antisense ODN (~35 mer), is observed in all the 4 lanes. No band of radioactivity is seen in the control mRNA samples (lanes 2, 4, 6, and 8) that were incubated with nonsense ODN, indicating the susceptibility of the unprotected radiolabeled ODN to S₁ nuclease digestion.

To assess the transcriptional and translational fibrillin-specific blocking activities of phosphorothioated antisense ODN,competitive PCR, immunoprecipitation, and immunofluorescence studieswere performed. The competitive RT-PCR method was chosen insteadof Northern blot analysis since only a minute amount total RNAcan be extracted from the E15 rat metanephric explant, i.e., ~0.6µg per explant. In both the nonsense (control) and antisense ODN-treatedgroups, a linearity in the ratio of wild to mutant fibrillin-1-DNAcould be maintained when plotted against 10² to 10⁷ serial logarithmic dilutions of the competitive template DNA(Fig. 6A). Within this range of dilution, the bands of wild-typeand mutant DNA were discernible for densitometric analyses tocalculate a ratio. A ratio of 1 was obtained at a dilution of10⁴ of the competitive DNA in explants of the nonsense ODN-treatedgroup (control). For the cDNA from explants treated with antisenseODN, a ratio of 1 was obtained at a dilution of 10⁶ with competitive DNA. However, for the $beta$ -actin, no significantdifferences in the linearity relationship, within the range of10¹ to 10⁶ dilutions of competitive DNA, or in the ratio of wild-type tomutant DNA were observed between the two groups (control and antisense)(Fig. 6B). These data suggest that the steady-state mRNA levelsof fibrillin-1 were selectively reduced with the exposure of metanephricexplants to antisense ODN, whereas that of the $beta$ -actin were unaffected.

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Fig. 6. Competitive RT-PCR of fibrillin-1 (A) and $beta$ -actin (B) cDNAs, prepared from sense/nonsense (control) and fibrillin-1 antisense ODN-treated kidney explants. Serial logarithmic dilutions of mutant competitive DNA template of fibrillin-1 and $beta$ -actin (see MATERIALS AND METHODS) were coamplified with a fixed amount (1 µl) of first-strand cDNA prepared from kidney explants. Amplified DNAs were subjected to 2% agarose gel electrophoresis, and densitometric tracings were prepared. Then, ratios between the densitometric readings of wild-type and mutant PCR products were plotted on logarithmic scales on the ordinate (y-axis) against the logarithmic dilutions of competitive DNA on the abscissa (x-axis). A ratio of 1 is obtained at a dilution of 10⁶ of the competitive DNA in the antisense ODN explant compared with the dilution of 10⁴ in the control explants. This indicates a reduction in the amplification of wild-type fibrillin-1 DNA in the antisense-treated kidney explants compared with the control (A). No differences in the amplification of $beta$ -actin between the two groups are observed (B).

For translational blockade studies, the antisense and sense/nonsense-treated metanephric explants were radiolabeled with [³⁵S]methionine, and extracts were immunoprecipitated with anti-fibrillin-1antibody and subjected to 5% SDS-PAGE. Under reducing conditions,extracts from the control untreated explants yielded a singleband of radioactivity with ~300-kDa size (Fig. 7D, lane 1). Nodecrease in the intensity of the band was observed in the extractsof the explants treated with sense/nonsense ODN (Fig. 7D, lane2). However, a marked decrease in the intensity of the band wasobserved in metanephric explants treated with the antisense ODN,even when double the amount of radioactivity, compared with thecontrols, was loaded for gel electrophoresis (Fig. 7D, lane 3).The tissue immunofluorescence studies confirmed the fibrillin-1translational blockade observed in the immunoprecipitation experiments.The control explants showed a normal population of the nascentnephrons and iterations of the ureteric bud branches (Fig. 7A).The immunoreactivities of the mesenchyme surrounding the developingnephrons could be well elucidated. No significant decrease inthe population of nephrons and the degree of anti-fibrillin-1immunoreactivity was observed in the explants treated with nonsenseODN (Fig. 7B). However, a remarkable decrease in the immunoreactivitywas observed in the explants treated with antisense ODN, and also,the population of the developing nephrons was also reduced (Fig.7C). In aggregate, both the immunofluorescence and the immunoprecipitationstudies indicated that the antisense ODN interferes with the translationof the fibrillin-1 gene.

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Fig. 7. A-C: immunofluorescence photomicrographs of the control untreated (A) and sense/nonsense- (B) and antisense-treated (C) explants, which were subsequently stained with anti-fibrillin-1 antibody. Untreated (A) and nonsense ODN-treated (B) explants reveal normal immunoreactivity of the mesenchyme surrounding the nascent nephrons (n) and ureteric bud branches (u). Antisense ODN-treated explant reveals a generalized reduced immunoreactivity with anti-fibrillin-1 antibody. D: SDS-PAGE autoradiogram of the extracts of the untreated (lane 1), nonsense ODN-treated (lane 2), and antisense ODN-treated explants (lane 3), which were immunoprecipitated with anti-fibrillin-1 antibody. A marked decrease in the autoradiographic intensity of the band in lane 3 is observed (large arrow), indicating that the translational blockade in the de novo synthesis of fibrillin-1 occurred as a result of antisense ODN treatment to the rat metanephric explants. Small arrow indicates the point of application.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

The results of this investigation indicate that the cDNA sequence of fibrillin-1 is highly conserved across human, mouse,and rat species. In the human sequence, a multitude of mutationsthroughout the entire open-reading frame of the fibrillin-1 cDNAis associated with Marfan syndrome (27). These mutations mayeither involve EGF- or cbEGF-like domains or latent TGF- $beta$ -bindingprotein motifs. However, most severe malformations are seen inmutations involving the central portion of the molecule, i.e.,a stretch between amino acid residue ~1050 to ~1350. Whether suchmutations can lead to defective fibril formation or perturb elastogenesisin mice and rats needs to be determined by transgenic or knockoutexperiments. Nevertheless, an internal duplication in the mousefibrillin-1 gene has been found to be associated with "tight skin"(Tsk) phenotype (37). The heterozygous Tsk mice exhibit cutaneousand skeletal abnormalities, whereas homozygous Tsk embryos diein utero due to failure in early organogenesis. In rat, so farno genetic mutation studies have been done. However, one may assumethat differences observed at the amino acid residues 416, 437,and 438 of fibrillin-1 between rat, mouse, and human are probablynot associated with any disease process, because the rat cDNAexhibiting deletion or addition at these sites has no abnormalphenotype in the rat. In addition, it is interesting to note that,although substitution of tyrosine at amino acid residue 2113 isseen in Marfan syndrome, in the rat this substitution (tyrosine $right-arrow$ phenylalanine) has no detectable phenotypicchange.

One would expect the role of fibrillin-1 in various biological processes to be common to all the mammalian species, becausethe putative protein's structural characteristics, i.e., conservedRGD sequence and cbEGF-like domains (Fig. 1), are similar. Fibrillinmay play a role in fibrillogenesis, elastogenesis, and vasculogenesis,processes in which it can confer biomechanical properties on avariety of connective tissues (24, 27, 29). In addition,because of the presence of cbEGF-like domains that mediate protein:proteininteractions, it may be involved in aggregation of macromoleculesor cells during early embryogenesis (8). Moreover, the RGDsequences that mediate anchorage dependence may further facilitatecell:matrix interactions prevalent during organogenesis in embryoniclife (16, 32, 34). Since fibrillins are also developmentallyregulated, this leads one to propose an emerging theme from theabove studies that they may play a vital role in embryogenesis.The finding that there is an increasing expression of fibrillin-1mRNA in rat fetal and neonatal renal tissues (Fig. 2) would supportthe notion that it, like other ECM proteins, plays a role in ratmetanephric development by acting as amorphogen.

A morphogen is defined as a molecule that expresses its concentration gradient in strategic locations of a given tissue andalters the fate of target cells in a dose-dependent manner (16).Given this definition, molecules other than ECM proteins, e.g.,protooncogenes, growth factors and their receptors, and ECM receptors,i.e., integrins, can be classified as morphogens (16, 25).Some of them are expressed in the mesenchyme, others in the epithelia,and still others at the epithelial:mesenchymal interface. Allthese diverse groups of molecules can conceivably participatein epithelial:mesenchymal interactions that are essential to themorphogenesis of various mammalian organs (16, 25). The epithelial:mesenchymalinteractions can be viewed as paracrine or juxtacrine interactions,where the ligand may be expressed in epithelium or mesenchyme,and the opposite would be the anticipated expression of the receptor.For instance the $alpha$ _v $beta$ ₃-integrin receptor is exclusively expressedin the ureteric bud epithelia and induced mesenchyme, whereasits ligands like fibronectin, vitronectin, type I and IV collagens,and laminin are present in the mesenchyme or at the epithelial:mesenchymalinterface (16, 40). Thus the fact that fibrillin-1 mediatesattachment of cells by the involvement of $alpha$ _v $beta$ ₃-integrin receptors(34) would suggest that, like $alpha$ _v $beta$ ₃, fibrillin-1 may be relevantin the organogenesis of the kidney. This notion is supported bythe fact that gene expression of fibrillin-1 is developmentallyregulated in strategic locations, i.e., the metanephric mesenchyme,as indicated by our in situ data (Fig. 3). Also, the fact thatprotein expression of fibrillin-1 is exclusively observed in themesenchyme during the early phase of metanephrogenesis and isdevelopmentally regulated, as well (Fig. 4), further strengthensthis notion. Here, one may suggest that fibrillin-1 could serveas a ligand for the $alpha$ _v $beta$ ₃-integrin receptor to mediate paracrineepithelial:mesenchymal interactions during metanephrogenesis.Indeed, such a suggestion has been made recently in studies inwhich it was evaluated whether fibrillin specifically interactswith the receptors or binding proteins on cells in tissues witha high expression of fibrillin (34).

In a manner similar to ligand:receptor ( $alpha$ _v $beta$ ₃:fibrillin-1) interaction in the early phases of mammalian metanephric developmentwhen epithelial:mesenchymal interactions are prevalent, fibrillinmay also modulate the later events like vascularization of thekidney. The fact that a rising gene as well as protein expressionof fibrillin, similar to that of $alpha$ _v $beta$ ₃ (40), was observed inthe vascular elements of the developing metanephros, i.e., arteriesand glomeruli (Figs. 3 and 4), suggests that it is likely thatit plays a role in the vascularization phase of the kidney. Insuch a role, one may envisage the involvement of "anchoring filaments"that have been identified in the subendothelial matrix of bloodvessels, where they connect the endothelia to the surroundingelastic fibers (34). These microfibrillar filaments containfibrillin, and they are anchored at the cell surface in the plasmalemmaldomains occupied by intracellular face membrane-associated denseplaques, sometimes referred to as focal contact points (34).Since $alpha$ _v $beta$ ₃ is known to associate into focal contacts to organizethe cytoskeletal assembly, there is a good possibility that thisintegrin receptor via its interactions with fibrillin modulatesthe later phases of metanephric development that are related tovascularization of the fetal kidney. The vascularization of themammalian kidney involves two interlinked processes, i.e., vasculogenesis(in situ blood vessel formation) and angiogenesis (sprouting ofpreexisting capillaries) (14). Both the processes are highlycomplex in nature and difficult to study in an organ culture system,and thus this study was restricted to elucidate the role of fibrillin-1in the early phases of metanephric developmentonly.

The role of fibrillin-1 in metanephric development was investigated by employing antisense ODN. The specificity of the ODNwas confirmed by subjecting RNA:DNA hybrids to S₁ nuclease digestion(Fig. 5), as described previously (17, 40). Also, the specificitywas maintained by using them at a relatively low concentration(0.5 µM) in in vitro conditions. Usually, the antisense or senseODNs have nonspecific translational inhibitory effects when usedabove a concentration of 1 µM in the medium (1). Moreover,at a higher concentration (>2.5 µM) they may be cytotoxic (1).However, at a relatively low concentration (<0.25 µM) the effectsin the target tissue may not be discernible, since they are readilysusceptible to nuclease degradation. The latter difficulty canbe overcome by employing phosphorothioated ODNs, which are quiteresistant to nuclease degradation (17, 40). The inclusionof phosphorothioated antisense ODN in the medium induced notablechanges in metanephroi. They included a reduced population ofnascent nephrons, disorganization of the ureteric bud iterations,and loss of the acuteness of their tips (Fig. 5). Such a lossof the acuteness of the tips of the ureteric bud branches hasbeen reported to perturb epithelial:mesenchymal interactions withultimate arrest in the formation of nascent nephrons (16). Themesenchyme is expanded, but the mesenchymal cells, toward whichthe fibrillin-1 antisense ODN is directed, seem to be quite atrophic.These observations suggest that fibrillin-1 induced perturbationin the biology of mesenchymal cells that led to an interferencein the epithelial:mesenchymal interaction and ultimately dysmorphogenesisof the metanephros. It is interesting to mention here that similardelayed morphogenesis of the rat metanephros has been reportedin experiments in which $alpha$ _v $beta$ ₃ antisense ODN was used (40), thussuggesting an interactive role of fibrillin-1 as a ligand and $alpha$ _v $beta$ ₃ as a receptor in metanephric development. The notion thatfibrillin-1 acts as a ligand for $alpha$ _v $beta$ ₃ has been well-documentedin cell culture studies (34). The specificity of the effectof fibrillin-antisense ODN was also supported by the gene expressionstudies, in which RT-PCR analyses were carried out (Fig. 6). Areduced mRNA expression of fibrillin-1 was observed, whereas nochange in the expression of $beta$ -actin was seen in the competitiveRT-PCR analyses with the antisense ODN treatment. Here, the questionof whether antisense ODN caused any translational blockade inthe de novo synthesis of fibrillin, which is ultimately responsiblefor dysmorphogenesis of the metanephric kidney, needs to be addressed.The fact that, along with the reduced mRNA levels, there was aconcomitant reduction in the immunoreactivity of anti-fibrillin-1antibody suggests that a decreased de novo synthesis of fibrillin-1has indeed occurred. Finally, the immunoprecipitation studiesconfirmed the translational blockade of fibrillin-1, in whicha notable decrease in the intensity of a ~300-kDa band was observedin the SDS-PAGE autoradiogram. Thus it is reasonable to proposethat the dysmorphogenesis of the metanephros is associated withgene-disruption of the ECM macromolecule, i.e., fibrillin-1.

In summary, this study reemphasizes the relevance of epithelial:mesenchymal/paracrine or juxtacrine interactions in rat metanephricdevelopment. Also, this investigation adds another ECM moleculeto our realm of knowledge, i.e., fibrillin-1, that seems to playa role in the organogenesis of the kidney, perhaps by acting asligand for $alpha$ _v $beta$ ₃ integrin, the latter being also a known receptorfor a well-established renal tubular morphogen, i.e., laminin(7).

	ACKNOWLEDGEMENTS

This work was supported by National Institute of Diabetes and Digestive and Kidney Diseases Grant DK-28492.

	FOOTNOTES

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: Y. S. Kanwar, Dept. of Pathology, Northwestern Univ. Medical School, 303 East Chicago Ave., Chicago, IL 60611.

Received 20 May 1998; accepted in final form 20 August 1998.

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