We accept PCR products straight off the thermal cycler for DNA purification before sequencing. We accept either individual PCR products in single tubes or 96-well plate format. 

Instead of purifying the PCR products straight off the PCR reaction, the unpurified PCR products are first run on an agarose gel, then the target DNA band is excised and purified using a silica gel extraction column kit.

We accept transformed bacterial cultures, grow them in our laboratory, and then extract the transformed plasmids using a plasmid prep kit prior to DNA sequencing. Now, we only accept stab culture for individual clones. 96-well format bacterial cultures are accepted in DNA pellet format on dry ice.

Before adding Ready-to-load samples into load into our Genetic Analyzer, we must add formamide or water into the samples. Residual ethanol on the precipitated BigDye® cycle sequencing will generate relatively low signal data. Hence, additional drying service is required for the customers who are not able to dry their purified BigDye® cycle sequencing reactions completely.

BigDye® cycle sequencing reaction is tolerant to contamination of RNase up to certain level. For DNA template that shows heavy RNA contamination of 1ug or more, it will show relatively low signal data in sequencing. RNase will be used to degrade excess RNA from the DNA template by incubation. Right after RNase treatment, the DNA template will be ethanol precipitated and purified before DNA sequencing.

This additional quantification service provides customers with a means of verifying and quantifying their DNA template prior to DNA sequencing. A small volume of DNA template is run on an agarose gel to verify its purity and mass before proceeding with DNA Sequencing reactions. 

This additional quantification service provides customers with a means of quantifying their DNA template prior to DNA sequencing. A small volume of DNA template is used to measure the concentration and optical density (OD) ratio of 260/280 using the Spectrophotometer.