anyone.. wondering if it really makes much difference versus "regular" ligase.

I use it and it works great for me (I can't make a comparison with regular ligase as I've used this as my sole ligase). What I can tell you is you get 400ul of the enzyme for ~$300, so it's not outrageously expensive.

so if you look at the details between the two SKUs the only difference is the concentration of the ligase and the "rapid" includes a buffer that has PEG in it (for molecular crowding).



The higher concentration is preferred for blunt-end ligations (since it's a lower efficiency reaction). However, for library construction we are ligating T-overhang adapters to A-overhang DNA fragments. The question this begs is why would we want to increase the efficiency of ligation between DNA fragments that don't have an A-overhang? And if it's correct (according to the Quail et al. paper) that the ligases from companies other than Enzymatics, have enough nuclease activity to convert some of the A-overhang fragments back into blunt end fragments then shouldn't we never use the rapid ligases?

Maybe someone has a cogent answer but I'm thinking I'm not going to use the "Quick/Rapid" ligases anymore (or just dilute them).

This is a common misconception. Blunt ligation is extremely efficient. In fact 1T:1A ligation is the trough in the efficiency plot (lower than both blunt and >1 base overhangs).

We've tried Enzymatics' "ultra-pure ligase". Compared to a lot of other ligases on the market there does seem to be a significant increase in ligated fragments as determined by qPCR pre and post ligation ( their ligase is what we currently use now). Utilizing Covaris for shearing also seemed to increase our ligation efficiencies.

I am in the purification department for enzymatics. Company purity standards are ten fold others. Nuclease activity is near nil.