Abstract

Extracellular matices have important roles in the morphogenesis and development of multicellular animals. Many extracellular matrix components have been identified, but in most cases little is known about the details of their assembly and function. The long-term goals of this proposal are to understand how extracellular matrix proteins assemble into organized macromolecular complexes and how these complexes function in morphogenesis and development. The most abundant and ubiquitous extracellular matrix proteins are the collagens. Several human connective tissue diseases have been shown to result from mutations in collagens. The powerful genetic and molecular analyses possible in the nematode C. elegans, and its well characterized anatomy and development make it an excellent system for studying collagen structure and function. Mutations in several cuticle collagen genes in C. elegans have profound effects on the animals morphogenesis. Many of these mutations have been shown to define a region involved in proteolytic processing. Antibodies will be used to examine the fates of unprocessed mutant collagens. The gene encoding the proteolytic enzyme will be identified, using the two hybrid system of yeast, and characterized. A second group of mutations are cysteine replacements in the carboxyl-terminal domains that affect both disulfide and tyrosine- based covalent bonding of the collagens. The function of the carboxyl domains in collagen assembly will be studied by analyzing site-directed mutations in transgenic animals, both phenotypically and with collagen- specific antibodies. The two-hybrid system will also be used to examine protein-protein interactions between collagen carboxyl domains. C. elegans collagens have been shown to be crosslinked with di- and (iso)trityrosine residues. The site of one of these crosslinks has been determined. This domain will be used to identify the enzyme responsible for tyrosine oxidation and crosslink formation, using assays for dityrosine formation as well as the two-hybrid system. Mutations of the enzyme will be generated, by PCR selection for transposon insertion, in order to determine the effects of reducing or eliminating crosslinking. Tyrosine crosslinks make nematode cuticles extremely tough and insoluble. An understanding of the mechanism of crosslink formation may lead to novel approaches for controlling parasitic nematodes, as well as valuable technical tools for manipulating C. elegans. The persistence of collagen mutant phenotypes from one developmental stage to the next, when the collagen gene is not expressed, was proposed to result from maintenance of the phenotype by the epidermal cytoskeleton. This proposal will be tested by expressing mutant collagens using regulatable promoters in transgenic animals, and determining if phenotypic persistence is observed in the manner predicted. These studies may reveal developmental interplay between the extracellular matrix and the cytoskeleton. The mutations that provided these insights into collagen function were selected because they exhibit unusual genetic interactions. Additional interacting mutations have and will be generated and analyzed, as they may identify novel extracellular matrix components and their important functional domains.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
Eunice Kennedy Shriver National Institute of Child Health & Human Development (NICHD)
Type
Research Project (R01)
Project #
5R01HD022028-11
Application #
2198420
Study Section
Pathobiochemistry Study Section (PBC)
Project Start
1986-08-01
Project End
1998-06-30
Budget Start
1995-07-01
Budget End
1996-06-30
Support Year
11
Fiscal Year
1995
Total Cost
Indirect Cost

  Institution

Name
Northwestern University at Chicago
Department
Anatomy/Cell Biology
Type
Schools of Dentistry
DUNS #
005436803
City
Chicago
State
IL
Country
United States
Zip Code
60611

  Publications

Yang, J; Kramer, J M (1999) Proteolytic processing of Caenorhabditis elegans SQT-1 cuticle collagen is inhibited in right roller mutants whereas cross-linking is inhibited in left roller mutants. J Biol Chem 274:32744-9
Bergmann, D C; Crew, J R; Kramer, J M et al. (1998) Cuticle chirality and body handedness in Caenorhabditis elegans. Dev Genet 23:164-74
Peixoto, C A; de Melo, J V; Kramer, J M et al. (1998) Ultrastructural analyses of the Caenorhabditis elegans rol-6 (su1006) mutant, which produces abnormal cuticle collagen. J Parasitol 84:45-9
Park, Y S; Kramer, J M (1994) The C. elegans sqt-1 and rol-6 collagen genes are coordinately expressed during development, but not at all stages that display mutant phenotypes. Dev Biol 163:112-24
Kramer, J M (1994) Genetic analysis of extracellular matrix in C. elegans. Annu Rev Genet 28:95-116
Yang, J; Kramer, J M (1994) In vitro mutagenesis of Caenorhabditis elegans cuticle collagens identifies a potential subtilisin-like protease cleavage site and demonstrates that carboxyl domain disulfide bonding is required for normal function but not assembly. Mol Cell Biol 14:2722-30
Levy, A D; Kramer, J M (1993) Identification, sequence and expression patterns of the Caenorhabditis elegans col-36 and col-40 collagen-encoding genes. Gene 137:281-5
Aroian, R V; Levy, A D; Koga, M et al. (1993) Splicing in Caenorhabditis elegans does not require an AG at the 3' splice acceptor site. Mol Cell Biol 13:626-37
Levy, A D; Yang, J; Kramer, J M (1993) Molecular and genetic analyses of the Caenorhabditis elegans dpy-2 and dpy-10 collagen genes: a variety of molecular alterations affect organismal morphology. Mol Biol Cell 4:803-17
Kramer, J M; Johnson, J J (1993) Analysis of mutations in the sqt-1 and rol-6 collagen genes of Caenorhabditis elegans. Genetics 135:1035-45

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