Repeat-primed PCR is the most common method for Fragile X syndrome (FXS) detection. A 38-bp insertion into 5'-UTR region of the FMR1 gene was noted to overestimate 13 repeats for the number of CGG repeats and present a discontinuous, atypical dragon's back peaks in repeat-primed PCR. The correct number of CGG repeats of this case was confirmed to be 67 by direct sequencing, instead of 80 by repeat-primed PCR. Although both number of CGG repeats were belonging to pre-mutation, their rates of full-mutation transition on fetus were greatly different, 5.3% and 57.8% for 67 and 80 CGG repeats, respectively. Higher full-mutation transition rate weights more in the following genetic counseling. To prevent excessive or even miss interpretation caused by incorrectly determining CGG repeats, DNA sequencing should be used to confirm CGG repeats while the discontinuous or interrupted atypical dragon's back peaks revealed in repeat-primed PCR.