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Dive into the research topics where Eija-Riitta Hämäläinen is active.

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Featured researches published by Eija-Riitta Hämäläinen.


Journal of Biological Chemistry | 1995

Quantitative Polymerase Chain Reaction of Lysyl Oxidase mRNA in Malignantly Transformed Human Cell Lines Demonstrates That Their Low Lysyl Oxidase Activity Is Due to Low Quantities of Its mRNA and Low Levels of Transcription of the Respective Gene

Eija-Riitta Hämäläinen; Ritva Kemppainen; Helena Kuivaniemi; Gerard Tromp; Antti Vaheri; Taina Pihlajaniemi; Kari I. Kivirikko

Lysyl oxidase (EC 1.4.3.13), an extracellular copper amino oxidase, initiates the cross-linking of collagens and elastin by catalyzing oxidative deamination of the -amino group in certain lysine and hydroxylysine residues. We developed here a polymerase chain reaction (PCR) method for the quantification of lysyl oxidase mRNA in which a synthetic RNA is used as an internal standard for coamplification with the targeted mRNA. The amount of lysyl oxidase mRNA when studied by Northern blot analysis and the number of lysyl oxidase mRNA molecules when determined by the quantitative PCR method were found to be markedly low in various malignantly transformed cell lines relative to control cell lines, quantitative PCR indicating values of about 2-10% of those in the controls. No difference was found in the number of β-actin mRNA molecules between the transformed cells and the controls. Nuclear runoff experiments indicated that most if not all of the decrease in the number of lysyl oxidase mRNA molecules can be explained by diminished transcription of the respective gene.


BMC Biotechnology | 2008

Improved production of human type II procollagen in the yeast Pichia pastoris in shake flasks by a wireless-controlled fed-batch system

Maria Ruottinen; Monika Bollok; Martin Kögler; Antje Neubauer; Mirja Krause; Eija-Riitta Hämäläinen; Johanna Myllyharju; Antti Vasala; Peter Neubauer

BackgroundHere we describe a new technical solution for optimization of Pichia pastoris shake flask cultures with the example of production of stable human type II collagen. Production of recombinant proteins in P. pastoris is usually performed by controlling gene expression with the strong AOX1 promoter, which is induced by addition of methanol. Optimization of processes using the AOX1 promoter in P. pastoris is generally done in bioreactors by fed-batch fermentation with a controlled continuous addition of methanol for avoiding methanol toxification and carbon/energy starvation. The development of feeding protocols and the study of AOX1-controlled recombinant protein production have been largely made in shake flasks, although shake flasks have very limited possibilities for measurement and control.ResultsBy applying on-line pO2 monitoring we demonstrate that the widely used pulse feeding of methanol results in long phases of methanol exhaustion and consequently low expression of AOX1 controlled genes. Furthermore, we provide a solution to apply the fed-batch strategy in shake flasks. The presented solution applies a wireless feeding unit which can be flexibly positioned and allows the use of computer-controlled feeding profiles.By using the human collagen II as an example we show that a quasi-continuous feeding profile, being the simplest way of a fed-batch fermentation, results in a higher production level of human collagen II. Moreover, the product has a higher proteolytic stability compared to control cultures due to the increased expression of human collagen prolyl 4-hydroxylase as monitored by mRNA and protein levels.ConclusionThe recommended standard protocol for methanol addition in shake flasks using pulse feeding is non-optimal and leads to repeated long phases of methanol starvation. The problem can be solved by applying the fed-batch technology. The presented wireless feeding unit, together with an on-line monitoring system offers a flexible, simple, and low-cost solution for initial optimization of the production in shake flasks which can be performed in parallel. By this way the fed-batch strategy can be applied from the early screening steps also in laboratories which do not have access to high-cost and complicated bioreactor systems.


Microbial Cell Factories | 2006

Optimisation of substrate feeding in shake flask cultures of Pichia pastoris for recombinant protein production

Monika Bollok; Maria Ruottinen; Mirja Krause; Antti Vasala; Eija-Riitta Hämäläinen; Antje Neubauer; Johanna Myllyharju; Peter Neubauer

who generously supported the meeting. Meeting abstracts - A single PDF containing all abstracts in this supplement is available he re . http://www. biomedcentral.co m/content/pdf/14 75-2859-5-S1-inf o.pdf


Genomics | 1991

Molecular cloning of human lysyl oxidase and assignment of the gene to chromosome 5q23.3-31.2

Eija-Riitta Hämäläinen; Tania A. Jones; Denise Sheer; Kirsi Taskinen; Taina Pihlajaniemi; Kari I. Kivirikko


Journal of Biological Chemistry | 2003

Assembly of Stable Human Type I and III Collagen Molecules from Hydroxylated Recombinant Chains in the Yeast Pichia pastoris EFFECT OF AN ENGINEERED C-TERMINAL OLIGOMERIZATION DOMAIN FOLDON

Outi Pakkanen; Eija-Riitta Hämäläinen; Kari I. Kivirikko; Johanna Myllyharju


Genomics | 1993

Structure of the human lysyl oxidase gene

Eija-Riitta Hämäläinen; Ritva Kemppainen; Taina Pihlajaniemi; Kari I. Kivirikko


Bio-medical Materials and Engineering | 2006

Cellulose sponge as a scaffold for cartilage tissue engineering

Hertta Pulkkinen; Virpi Tiitu; Eveliina Lammentausta; Mikko S. Laasanen; Eija-Riitta Hämäläinen; Ilkka Kiviranta; Mikko J. Lammi


International Journal of Artificial Organs | 2008

Recombinant human type II collagen as a material for cartilage tissue engineering.

Hertta Pulkkinen; Virpi Tiitu; Piia Valonen; Eija-Riitta Hämäläinen; Mikko J. Lammi; Ilkka Kiviranta


Archives of Biochemistry and Biophysics | 1996

Expression of mRNAs for Lysyl Oxidase and Type III Procollagen in Cultured Fibroblasts from Patients with the Menkes and Occipital Horn Syndromes as Determined by Quantitative Polymerase Chain Reaction

Ritva Kemppainen; Eija-Riitta Hämäläinen; Helena Kuivaniemi; G. Tromp; Taina Pihlajaniemi; Kari I. Kivirikko


Journal of Investigative Dermatology | 1996

Quantification of Proα1(I) Collagen mRNA in Skin Biopsy Specimens: Levels of Transcription in Normal Skin and in Granuloma Annulare

Kaisa Tasanen; Eija-Riitta Hämäläinen; Riitta Palatsi; Aarne Oikarinen

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Peter Neubauer

Technical University of Berlin

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