I am working on RNAi of nematode genes for which I am adopting gateway cloning strategies. In this strategy to clone the gene in the entry vector (I am using pDONR221 from invitrogen) some adapter sequence (att B1 & B2) has to be added in our gene of interest. The only way to add those sequences in the upstream of forward (attB1) and reverse primer (attB2) before going for PCR. The problem I faced while designing the primer was invitrogen provided the sequence of attB1 is GGGGACAAGTTTGTACAAAAAAGCAGGCT. But when I checked in oligocalc software (http://www.basic.northwestern.edu/biotools/oligocalc.html) this one showed there is a potential of hairpin formation and self annealing site. so I am worried PCR may not work. Also primer length is going to be too high 29+20 bp (attB+gene specific) leading to high annealing temperature. Does anyone have any suggestions?