There are several things you could try:
1. Hit the flasks. I’m serious. If you’ve never tried it, it is definitely worth to try. Nothing bad can happen, so hit away. In my experience it is best to hit it from the side, so cells won’t fly into the tip of the flask.
2. Leave them with the trypsin a little longer in the incubator. Not too long though, you might end killing them.
3. How exactly do you count them? When i used to count cells i first inactivated the trypsin with growth medium, then take the whole thing and put in the centrifuge, then throw away the medium+trypsin and resuspend in a buffer such as PBS. Then you can try to further break down the clumps by rapidly pipetting in and out with an automatic pipette. I used to do this with a 100-1000 pipette, but then again i never had any problem. You could use a 20-200 pipette set on 200 because the tip is much narrower. If all else fails, that might solve your problem.
4. If the clumps are small, leave them as is. The counting chamber has a huge error anyway.
5. I just thought of this, no idea if it would work: what about putting the cells in a Corning tube and vortexing them? There might be a speed big enough to break them apart without killing them.

Anyway, let me know what you end doing to solve the problem.