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Featured researches published by Íñigo Santamaría.


Journal of Biological Chemistry | 2002

Structural and Enzymatic Characterization of Drosophila Dm2-MMP, a Membrane-bound Matrix Metalloproteinase with Tissue-specific Expression

Elena Llano; Géza Ádám; Alberto M. Pendás; Víctor Quesada; Luis M. Sánchez; Íñigo Santamaría; Stéphane Noselli; Carlos López-Otín

We report the isolation and characterization of a cDNA encoding Dm2-MMP, the second matrix metalloproteinase (MMP) identified in the Drosophila melanogaster genome. The cloned cDNA codes for a polypeptide of 758 residues that displays a domain organization similar to that of other MMPs, including signal peptide, propeptide, catalytic, and hemopexin domains. However, the structure of Dm2-MMP is unique because of the presence of an insertion of 214 amino acids between the catalytic and hemopexin domains that is not present in any of the previously described MMPs. Dm2-MMP also contains a C-terminal extension predicted to form a cleavable glycosylphosphatidylinositol anchor site. Western blot and immunofluorescence analysis of S2 cells transfected with the isolated cDNA confirmed that Dm2-MMP is localized at the cell surface. Production of the catalytic domain of Dm2-MMP inEscherichia coli and analysis of its enzymatic activity revealed that this proteinase cleaves several synthetic peptides used for analysis of vertebrate MMPs. This proteolytic activity was abolished by MMP inhibitors such as BB-94, confirming that the isolated cDNA codes for an enzymatically active metalloproteinase. Reverse transcription-PCR analysis showed thatDm2-MMP is expressed at low levels in all of the developmental stages of Drosophila as well as in adult flies. However, detailed in situ hybridization at the larval stage revealed a strong tissue-specific expression in discrete regions of the brain and eye imaginal discs. According to these results, we propose that Dm2-MMP plays both general proteolytic functions during Drosophila development and in adult tissues and specific roles in eye development and neural tissues through the degradation and remodeling of the extracellular matrix.


Journal of Biological Chemistry | 1999

Molecular Cloning and Structural and Functional Characterization of Human Cathepsin F, a New Cysteine Proteinase of the Papain Family with a Long Propeptide Domain

Íñigo Santamaría; Gloria Velasco; Alberto M. Pendás; Ana Paz; Carlos López-Otín

A cDNA encoding a new cysteine proteinase belonging to the papain family and called cathepsin F has been cloned from a human prostate cDNA library. This cDNA encodes a polypeptide of 484 amino acids, with the same domain organization as other cysteine proteinases, including a hydrophobic signal sequence, a prodomain, and a catalytic region. However, this propeptide domain is unusually long and distinguishes cathepsin F from other proteinases of the papain family. Cathepsin F also shows all structural motifs characteristic of these proteinases, including the essential cysteine residue of the active site. Consistent with these structural features, cathepsin F produced in Escherichia coli as a fusion protein with glutathione S-transferase degrades the synthetic peptide benzyloxycarbonyl-Phe-Arg-7-amido-4-methylcoumarin, a substrate commonly used for functional characterization of cysteine proteinases. Furthermore, this proteolytic activity is blocked bytrans-epoxysuccinyl-l-leucylamido-(4-guanidino)butane, an inhibitor of cysteine proteinases. The gene encoding cathepsin F maps to chromosome 11q13, close to that encoding cathepsin W. Cathepsin F is widely expressed in human tissues, suggesting a role in normal protein catabolism. Northern blot analysis also revealed a significant level of expression in some cancer cell lines opening the possibility that this enzyme could be involved in degradative processes occurring during tumor progression.


Cancer Research | 1998

Cathepsin L2, a Novel Human Cysteine Proteinase Produced by Breast and Colorectal Carcinomas

Íñigo Santamaría; Gloria Velasco; Maite Cazorla; Antonio Fueyo; Elias Campo; Carlos López-Otín


Journal of Biological Chemistry | 1998

Cathepsin Z, a Novel Human Cysteine Proteinase with a Short Propeptide Domain and a Unique Chromosomal Location

Íñigo Santamaría; Gloria Velasco; Alberto M. Pendás; Antonio Fueyo; Carlos López-Otín


Molecular Biology of the Cell | 2005

Carbohydrate- and conformation-dependent cargo capture for ER-exit

Christian Appenzeller-Herzog; Beat Nyfeler; Peter Burkhard; Íñigo Santamaría; Carlos López-Otín; Hans-Peter Hauri


Genomics | 1996

Fine physical mapping of the human matrix metalloproteinase genes clustered on chromosome 11q22.3.

Alberto M. Pendás; Íñigo Santamaría; Alvarez Mv; Pritchard M; Carlos López-Otín


Kidney International | 2003

Influence of polymorphisms in VDR and COLIA1 genes on the risk of osteoporotic fractures in aged men

Daniel Álvarez-Hernández; Manuel Naves; J.Bernardino Diaz-lópez; Carlos Gómez; Íñigo Santamaría; Jorge B. Cannata-Andía


The Lancet | 1997

Prostate-specific membrane antigen in breast carcinoma.

José A. Uría; Gloria Velasco; Íñigo Santamaría; Adolfo A. Ferrando; Carlos López-Otín


Kidney International | 2003

Response of parathyroid glands to calcitriol in culture: Is this response mediated by the genetic polymorphisms in vitamin D receptor?

Daniel Álvarez-Hernández; Manuel Naves; Íñigo Santamaría; Javier Menárguez; Vicente Torregrosa; J.B. Cannata


Mutagenesis | 1994

The w/w+ SMART is a useful tool for the evaluation of pesticides

Ignacio Aguirrezabalaga; Íñigo Santamaría; Miguel A. Comendador

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Alberto M. Pendás

Spanish National Research Council

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Javier Menárguez

Complutense University of Madrid

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