Real-time determination of telomerase activity in cell extracts using an optical biosensor

Real-time determination of telomerase activity in cell extracts using an optical biosensor

A biosensoric approach has been developed to determine the activity of telomerase in tumor cell lysates. An optical sensor, the grating coupler, was used to monitor the association and dissociation of unlabeled compounds on the sensor surface in real time, by virtue of an evanescent field. An oligon...

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Bibliographic Details
Published in:Biological chemistry Vol. 383; no. 10; p. 1659
Main Authors: Schmidt, Peter M, Matthes, Eckart, Scheller, Frieder W, Bienert, Michael, Lehmann, Christine, Ehrlich, Angelika, Bier, Frank F
Format: Journal Article
Language:English
Published: Germany 01-10-2002
Subjects:
Base Sequence
Biosensing Techniques - instrumentation
Biosensing Techniques - methods
Buffers
Cell Extracts - analysis
Fibroblasts - enzymology
HL-60 Cells
Humans
Kinetics
Molecular Sequence Data
Oligonucleotides - chemistry
Oligonucleotides - genetics
Optics and Photonics - instrumentation
Peptide Nucleic Acids - pharmacology
Protein Binding
Sensitivity and Specificity
Surface Properties
Telomerase - chemistry
Telomerase - metabolism
Tumor Cells, Cultured
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Summary:A biosensoric approach has been developed to determine the activity of telomerase in tumor cell lysates. An optical sensor, the grating coupler, was used to monitor the association and dissociation of unlabeled compounds on the sensor surface in real time, by virtue of an evanescent field. An oligonucleotide was immobilized on the surface of the optical biosensor and linked with two other oligonucleotides by complementary sequences in an overlapping manner. The 3'-end of the last one carried the sequence of the telomeric substrate (TS) primer used for elongation by telomerase in the telomeric repeat amplification protocol (TRAP) assay. This primer sequence was phosphorothioate (PS)-modified, which is known to strongly increase the affinity to the primer binding site of telomerase protein and consequently the velocity of the telomerase reaction. We show that the PS primer binds to the modified biosensor and is elongated effectively by the telomerase from HL-60 cell lysates. A synthesis rate of 1 nucleotide/min was determined. The inhibitory effect of peptide nucleic acid (PNA) was shown by using immobilized TS. The velocity of the telomerase reaction was slowed down and the signal intensity was below the signal-to-noise ratio. Most nucleic acid detection systems use amplification steps such as polymerase chain reaction (PCR) to increase the amount of the probe. Since telomerase is a polymerase itself amplification of DNA by PCR is not required. Furthermore, no purification steps were required since all measurements were performed with crude cell extract.
ISSN:1431-6730
DOI:10.1515/BC.2002.186