Synthesis and Applications of Chemical Probes for Human O6-Alkylguanine-DNA Alkyltransferase

## Abstract Novel radiolabeled O^6^‐benzylguanine derivatives, 2‐amino‐6‐O‐[^11^C]‐[(methoxymethyl)benzyloxy]‐9‐benzyl purines ([^11^C]__p__‐O^6^‐AMBP, **1a**; [^11^C]__m__‐O^6^‐AMBP, **1b**; [^11^C]__o__‐O^6^‐AMBP, **1c**), have been synthesized for evaluation as new potential positron emission to

## Abstract __O^6^__‐alkylguanine‐DNA alkyltransferase (AGT) plays an important role in the repair of __O^6^__‐alkylguanine adducts, which are major mutagenic lesions produced by environmental carcinogens. Polymorphisms in the __AGT__ gene may affect the capacity to repair DNA damage and thereby ha

O 6 -Alkylguanine-DNA-alkyltransferase (ATase) is an important modulator of alkylating agent-induced toxicity and carcinogenicity, but those factors which influence the expression of this repair protein in human tissues are poorly characterised. In this study, we have determined ATase levels in macr

## Abstract O^6^‐alkylguanine‐DNA alkyltransferase (AGT) is mainly responsible for tumour resistances observed in chemotherapeutic treatments by chloroethylnitrosoureas (CENUs). Measurement of AGT activity is thereby essential to predict the response of the patients to therapy with CENUs. In order

## Extracts of three of the hepatitis-B liver samples containing 20 The principal carcinogenic and toxic lesion produced in mg of total protein, varying amounts of pure recombinant human ATase protein, and molecular weight markers (Amersham Interna-DNA by N-nitrosocompounds is likely to be O 6 -al