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Featured researches published by Walter Märki.


FEBS Journal | 1991

Alpha-factor-leader-directed secretion of recombinant human-insulin-like growth factor I from Saccharomyces cerevisiae. Precursor formation and processing in the yeast secretory pathway.

Klaus Steube; Bhabatosh Chaudhuri; Walter Märki; James P. Merryweather; Jutta Heim

A synthetic gene coding for human-insulin-like growth factor I (IGFI) was fused to the leader sequence of yeast prepro-alpha-factor and expressed in Saccharomyces cerevisiae under the control of a glyceraldehyde-3-phosphate dehydrogenase promoter fragment. Recombinant IGFI was found inside yeast cells and secreted into the medium. The secreted IGFI migrated on SDS gels with the same electrophoretic mobility as authentic IGFI, i.e. at about 7.5 kDa. HPLC analysis of secreted IGFI revealed the presence of the correctly folded, genuine molecule as well as an isomeric byproduct of equal molecular mass but with two of the three disulfide bonds interchanged. Inside exponentially growing cells the 7.5-kDa IGFI was also found, along with up to four additional IGFI-related polypeptides of higher molecular mass. By endoglycosidase F treatment the three polypeptides between 19-26 kDa were converted to a single peptide of 17 kDa. Since this peptide also reacted with an anti-alpha-factor antibody, it represents most likely the unglycosylated alpha-factor--IGFI fusion precursor. Pulse-chase experiments established the precursor nature of the intracellular higher-molecular-mass IGFI species. Conversion of the primary translation product to the differently glycosylated IGFI precursor proteins and into the mature form occurred very rapidly, within 2 min. Rapid maturation was, however, not followed by an equally rapid secretion of the mature form into the medium: only after 30-40 min did IGFI appear outside the cells. We therefore postulate the presence of an as yet undefined Golgi or post-Golgi bottleneck representing a major obstacle in secretion of recombinant IGFI from S. cerevisiae cells.


Nucleosides, Nucleotides & Nucleic Acids | 1985

A Large Fragment Approach to Gene Synthesis

Hans Rink; Manfred Liersch; Peter Sieber; Walter Märki; P. Meyer

Abstract The total synthesis of a 232 base-pair coding sequence of the proteinase inhibitor eglin c from only six synthetic fragments is described.


FEBS Journal | 1987

Stereospecific assignments of side-chain protons and characterization of torsion angles in Eglin c

Sven G. Hyberts; Walter Märki; Gerhard Wagner


The Journal of Antibiotics | 1990

Duramycins B and C, two new lanthionine containing antibiotics as inhibitors of phospholipase A2 : structural revision of duramycin and cinnamycin

Andreas Fredenhagen; Gabriele Fendrich; Fritz Märki; Walter Märki; Johannes Gruner; Fritz Raschdorf; Heinrich Peter


Thrombosis and Haemostasis | 1990

The anticoagulant and antithrombotic properties of hirudins.

Walter Märki; Robert B. Wallis


Archive | 1985

Process for the preparation of thrombin inhibitors

Manfred Liersch; Hans Rink; Walter Märki; Markus Grütter; Bernd Meyhack


FEBS Journal | 1994

C-Terminal Proteolytic Degradation of Recombinant Desulfato-Hirudin and Its Mutants in the Yeast Saccharomyces cerevisiae

Jutta Heim; Kenji Takabayashi; Bernd Meyhack; Walter Märki; Gabriele Pohlig


Seminars in Thrombosis and Hemostasis | 1991

Recombinant hirudin: genetic engineering and structure analysis.

Walter Märki; Hugo Grossenbacher; Markus Grütter; Manfred Liersch; Bernd Meyhack; Jutta Heim


Archive | 1986

Production of thrombin inhibitors

Bernd Meyhack; Walter Märki; Jutta Heim


Journal of Mass Spectrometry | 1996

Characterization of a β‐Asp33 Isoform of Recombinant Hirudin Sequence Variant 1 by Low‐energy Collision‐induced Dissociation

Patrick Schindler; Dieter Müller; Walter Märki; Hugo Grossenbacher; Wilhelm J. Richter

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