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Merck
CN
  • Microfluidic chip coupled with modified paramagnetic particles for sarcosine isolation in urine.

Microfluidic chip coupled with modified paramagnetic particles for sarcosine isolation in urine.

Electrophoresis (2013-06-19)
Ondrej Zitka, Natalia Cernei, Zbynek Heger, Miroslav Matousek, Pavel Kopel, Jindrich Kynicky, Michal Masarik, Rene Kizek, Vojtech Adam
摘要

Carcinoma of prostate (CaP) is the second most frequent malignant tumor occurring in men in Europe. Currently there is discussion on a wide range of potential CaP markers.One of them—nonprotein amino acid sarcosine, also known as N-methylglycine was chosen as a challenge for the development of microfluidic system with isolation by modified paramagnetic microparticles. Therefore, the aim of this study was to design a low-cost, simple, and rapid microfluidic system based on sarcosine isolation with modified paramagnetic microparticles and subsequent analysis on the ion exchange LC. We modified Dowex microparticles with Fe2O3 nanoparticles. Our paramagnetic microparticles were able to establish the binding with sarcosine. Moreover, we designed microfluidic device for sarcosine determination. Analysis of samples was carried out with LOD of1 M of a sarcosine that is sufficient because it is similar to concentrations of a sarcosine observed in the CaP patients.Carcinoma of prostate (CaP) is the second most frequent malignant tumor occurring in men in Europe. Currently there is discussion on a wide range of potential CaP markers.One of them—nonprotein amino acid sarcosine, also known as N-methylglycine was chosen as a challenge for the development of microfluidic system with isolation by modified paramagnetic microparticles. Therefore, the aim of this study was to design a low-cost, simple, and rapid microfluidic system based on sarcosine isolation with modified paramagnetic microparticles and subsequent analysis on the ion exchange LC. We modified Dowex microparticles with Fe2O3 nanoparticles. Our paramagnetic microparticles were able to establish the binding with sarcosine. Moreover, we designed microfluidic device for sarcosine determination. Analysis of samples was carried out with LOD of1 M of a sarcosine that is sufficient because it is similar to concentrations of a sarcosine observed in the CaP patients.

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Sigma-Aldrich
肌氨酸, 98%
Sigma-Aldrich
肌氨酸, BioXtra
Sigma-Aldrich
肌氨酸, crystallized, ≥98.0% (T)