Hi Laruo,

I think the reason why they don't suggest a Bioanalyzer after fragmentation is because they optimized the protocol for two specific insert sizes - 350 and 550 bp.

If your DNA is good, there shouldn't be any problems with the fragmentation if you use the parameters that they suggest. If you are still unsure about it, I think you can just take 1 µl of sheared DNA (of the 52.5 µl from the Covaris tube) and run it on a HighSensitivity Bioanalyzer chip.
On general, you can always test your shearing beforehand by not doing an Illumina library, but just shearing your DNA and then checking it with the Bioanalyzer or a normal gel.

Illumina mentions all the safe stopping points in their protocol where you can freeze (-20ºC) the library and continue some other day:
1) after end repair and size selection
2) after adapter ligation
3) after PCR
be sure to perform the necessary clean-up steps before you freeze the library.