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Highly Efficient Labeling of DNA Polymerases by a Binary System of Photoaffinity Reagents

N. A. Lebedeva*, D. M. Kolpashchikov, N. I. Rechkunova, S. N. Khodyreva, and O. I. Lavrik

Novosibirsk Institute of Bioorganic Chemistry, Siberian Division of the Russian Academy of Sciences, pr. Lavrent'eva 8, Novosibirsk, 630090 Russia; fax: (3832) 333-677; E-mail: nataleb@niboch.nsc.ru

* To whom correspondence should be addressed.

Received June 12, 2001; Revision received February 5, 2002
A binary system of photoaffinity reagents was proposed earlier for highly efficient labeling of DNA polymerases by 5´-[32P]DNA primers. In the present study we demonstrate the feasibility of this approach to increase the efficiency of DNA polymerase labeling. A photoactive 2,3,5,6-tetrafluoro-4-azidobenzoyl (FAB) group was incorporated at the 3´-end of 5´-[32P]DNA primers synthesized by DNA polymerase beta or Tte in the presence of one of the dTTP analogs--FAB-4-dUTP, FAB-9-dUTP, or FAB-4-ddUTP. The reaction mixture was irradiated by light with wavelength of 334-365 nm (direct labeling) or 365-450 nm in the presence of photosensitizer, one of dTTP analogs containing a pyrene moiety, Pyr-6-dUTP or Pyr-8-dUTP. In the case of the binary system of photoaffinity reagents, a FAB group is activated by energy transfer from sensitizer localized in the dNTP-binding site of DNA polymerase in the triple complex, comprised by reagent, DNA polymerase, and Pyr-6(8)-dUTP. Direct activation of the FAB group under these conditions is negligible. The most efficient photolabeling of DNA polymerases was observed with a primer containing a FAB-4-dUMP group at the 3´-end, and Pyr-6-dUTP as a photosensitizer. Using 10-fold molar excess of photoreagent to DNA polymerase beta, the labeling efficiency was shown to achieve 60%, which is 2-fold higher than the efficiency of the direct DNA polymerase labeling under harsher conditions (334-365 nm).
KEY WORDS: photoaffinity labeling, photoreactive dNTP analogs, binary system of photoaffinity reagents