Hi,

Actually we prepared library for 16s for illumina miseq got good amount of amplification but we dint compare with the primer without the illumina tags. now i think from your question that we should once compare both.

dear clmcmurray,

Yes, when ever you use fusion-primers you suck efficiency out of the PCR and this can have a lot of impact on low-template samples. My advice would be to use standard and fusion primers and run both on qPCR (with sybr) to see how much of a 'shift' you are getting. And see how much input template you can put into your reaction before it becomes a problem (i.e you run out or it is inhibitory).

One option is to do the fusion PCR and spike in 10% of standard primer - this may help your PCR get off the ground (these products will not cluster downstream)

The last option is to use a ligation based approach to library build.

There is strengths and weaknesses to each of these approaches - best of luck.