Met-ase: cloning and distinct chromosomal location of a serine protease preferentially expressed in human natural killer cells

Met-ase: cloning and distinct chromosomal location of a serine protease preferentially expressed in human natural killer cells

A cDNA clone encoding a human NK serine protease was obtained by screening a lambda-gt10 library from the Lopez NK leukemia with the rat natural killer Met-ase (RNK-Met-1) cDNA clone. In Northern blot analysis human Met-ase (Hu-Met-1) cDNA hybridized with a 0.9-kb mRNA in two human NK leukemia cell...

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Veröffentlicht in:The Journal of immunology (1950) 1993-12, Vol.151 (11), p.6195-6205
Hauptverfasser: Smyth, MJ, Sayers, TJ, Wiltrout, T, Powers, JC, Trapani, JA
Format: Artikel
Sprache:eng
Schlagworte:
Amino Acid Sequence
Animals
Base Sequence
BASIC BIOLOGICAL SCIENCES
Biological and medical sciences
BIOLOGICAL MATERIALS
BLOOD
BLOOD CELLS
BODY FLUIDS
cDNA
Chromosome Mapping
CHROMOSOMES
Chromosomes, Human, Pair 19
CLONING
Cloning, Molecular
DNA HYBRIDIZATION
DNA SEQUENCING
DNA, Complementary - isolation & purification
DNA-CLONING
ENZYMES
Fundamental and applied biological sciences. Psychology
GENE REGULATION
GENES
Genes. Genome
GENETIC MAPPING
Hu-Met-1 gene
HUMAN CHROMOSOME 19
HUMAN CHROMOSOMES
Humans
HYBRIDIZATION
HYDROLASES
Killer Cells, Natural - enzymology
LEUKOCYTES
man
MAPPING
MATERIALS
Molecular and cellular biology
Molecular genetics
Molecular Sequence Data
NATURAL KILLER CELLS
nucleotide sequence
ORGANIC COMPOUNDS
PEPTIDE HYDROLASES
predictions
PROTEINS
Rats
RNA, Messenger - analysis
Serine Endopeptidases - chemistry
Serine Endopeptidases - genetics
serine proteinase
SERINE PROTEINASES
STRUCTURAL CHEMICAL ANALYSIS 550400 > Genetics
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Zusammenfassung:A cDNA clone encoding a human NK serine protease was obtained by screening a lambda-gt10 library from the Lopez NK leukemia with the rat natural killer Met-ase (RNK-Met-1) cDNA clone. In Northern blot analysis human Met-ase (Hu-Met-1) cDNA hybridized with a 0.9-kb mRNA in two human NK leukemia cell lines, unstimulated human PBMC, and untreated purified CD3-CD56+ large granular lymphocytes. Unlike other members of the granzyme family that are highly expressed in activated peripheral T cells, the Hu-Met-1 transcript was barely detected in a population of PMA and ionomycin or IL-2-treated high density T cells. Several in vitro cultured Burkitt lymphomas, chronic- and promyeloid leukemias, acute lymphoblastic leukemias, and colon and ovarian carcinomas and colon and ovarian carcinomas did not express Hu-Met-1 mRNA. Hu-Met-1 mRNA expression in a small number of human T cell tumor lines did not correlate with any particular phenotype or stage of development. The presence of Hu-Met-1 mRNA closely correlated with the Met-ase activity of cellular lysates prepared from these various human peripheral blood subsets and in vitro cultured cell lines. Met-ase activity detected in whole cell lysates of cytotoxic lymphocytes was associated with the cytoplasmic granules of these cells. The nucleotide sequence of the Hu-Met-1 cDNA clone encodes a predicted serine protease of 257 amino acids. The predicted protein is an active enzyme of 232 amino acids with a calculated unglycosylated m.w. of 27,100. Hu-Met-1 is 66% identical to RNK-Met-1 at the amino acid level. The human and rat mature protein sequences conserve the active site His, Asp, and Ser amino acids that form the catalytic triad of serine proteases, all 8 cysteine residues, and several amino acids critical in the formation of the substrate binding pocket. The gene for the Hu-Met-1 serine protease is located on chromosome 19, which distinguishes it from any other member of the human granzyme family.
ISSN:0022-1767
1550-6606
DOI:10.4049/jimmunol.151.11.6195