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Sensors and Materials
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Sensors and Materials, Volume 16, Number 8 (2004)
Copyright(C) MYU K.K.
pp. 401-412
S&M577 Research Paper of Special Issue
Published: 2004

Development of a tRNA-Synthetase Microarray for Protein Analysis [PDF]

Qinglai Meng, Michael Mecklenburg, Bengt Danielsson, Klas Risveden and Bin Xie

(Received July 17, 2004; Accepted November 24, 2004)

Keywords: microarray, aminoacyl-tRNA synthatases (aaRS), glutamyl-tRNA synthetase (GluRS), microfluidics, XNA on GoldTM, protein analysis

Proteins are composed of 20 different amino acids. In the translation process, each of these 20 amino acids is specifically recognized by their cognate aminoacyl-tRNA syn- thetase. The fidelity of this recognition system is essential if translation is to function properly. The development of an in vitro system based on this recognition scheme would make a powerful analytical tool with which to analyse translation, as well as providing an additional biomimetic scheme for protein analysis. Aminoacyl-tRNA synthetases microarrays could be applied to protein fingerprinting and sequence analysis. The fabrica- tion of aminoacyl-tRNA synthetase arrays requires the use of advanced protein arraying technology that has only recently become available. In order to demonstrate the feasibility of this scheme, glutamyl-tRNA synthetase (GluRS) was immobilized on the streptavidin- based XNA on GoldTM biochip platform. The streptavidin layer provides a simple, efficient immobilization scheme that reduces nonspecific binding and improves the biocompatibility of the surface. Here, we demonstrate that biotinylated GluRS can be successfully immobi- lized on XNA on GoldTM. The immobilization efficiency was determined by double labelling GluRS with biotin and the fluorescent label Cy5. The CCD fluorescent micros- copy images revealed that the GluRS was efficiently immobilized and evenly distributed over the surface. Control experiments indicate a very low degree of nonspecific binding which is essential if detection of these multicomponent, low-affinity interactions is to be realized. Furthermore, we show that immobilization does not significantly reduce the function of the enzyme. In addition to the specific aims of this study, this technology would provide valuable insights into the biomechanics of translation as well as being a tool for studying tRNA modifications and subclasses. Moreover, the implications for develop- ing coupled transcription and translation systems should not be overlooked. Protein analysis schemes based on this approach would provide an urgently needed compliment to traditional methods. Finally, these arrays might also be useful tools in our efforts to understand the regulatory functions that small RNAs, i.e., iRNA, have been shown to play.

Corresponding author: Bin Xie


Cite this article
Qinglai Meng, Michael Mecklenburg, Bengt Danielsson, Klas Risveden and Bin Xie, Development of a tRNA-Synthetase Microarray for Protein Analysis, Sens. Mater., Vol. 16, No. 8, 2004, p. 401-412.



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