Single-stranded DNA binding proteins isolated from mouse brain recornize specific trinucleotide repeat sequencesin vitro

Abstract

Expansion of trinucleotide repeats (CAG)_n and (CGG)_n is found in genes responsible for certain human hereditary neurodegenerative diseases. By gel-mobility shift assay, we detected a single-stranded (AGC)_n repeat-binding activity primarily In mouse brain extracts and very low or undetectable activity in other tissue extracts. Two (AGC)_n-repeat binding proteins, with apparent molecular weights of 44 and 40 kDa, have been purified from mouse adult brain by a DNA affinity column and fast protein liquid chromatography. UVcross linking of radioiabeled (AGC)_n repeats with crude brain extracts and with purified two proteins of 44 and 40 kDa produced identical doublet bands, indicating that these proteins are In fact responsible for the (AGC)n-binding activity in brain extracts. We designated these two proteins TRIP-1 for the 44 kDa protein and TRIP-2 for the 40 kDa protein, where TRIP represents trinucleotide repeat-binding protein. TRIP-1 and TRIP-2 bind to a specific subset of trinucleotide repeat sequences including (AGC)_n, (AGT)_n, (GGC)_n, and (GGT)_n repeats but not to various other trinucleotide repeats. A minimum of eight (AGC) trinucleotide repeating units is required for TRIP-1 and -2 recognition and binding. The (AGC)_n repeat-binding activity increases In the brain after birth and reaches a plateau within 3 weeks. In the brain, TRIP-1 and TRIP-2 may alter the function of the genes containing the xpandedtrinucleotide repeats.