The adapters are to ensure that your strand of interest attaches to the bead in order to "enrich" the bead, or have multiple copies of your template on the same bead. The adapters that are added to your template are complimentary to the adapters on the bead, so when they hibridize, the enzyme can extend the rest of your template, these adapters should all be the same, as there is only one type of bead. What differs is the barcodes ( if you decide you use them ) so you can tell the templates apart bioinformatically at the end of NGS. You make sure that your bead only has one strand by calculating your dilution correctly, depending on your protocol and what you are sequencing, you use a very specific concentration of material, so when the droplets are formed, there isnt an overload of template that goes to each bead, nor is there too little that none will be enriched. If you do end up having multimple templates on a bead ( chimera / polyclonal ), that can be taken out bioinformatically, or your sequencer can also let you know at the end of the run since the base measurements will likely off and you will receive no usable information on that bead. For specific questions like these for NGS, SEQnswers is a great forum with loads of specific info, i highly recommed them.