Thank you all the colleagues that reached out in person and via DMs to share their thoughts, organisers for giving me the opportunity and amazing chair Martha Ingola and @mtrost.bsky.social

🤷‍♂️ the company rep says you can reuse them and we’ve had a good experience working with 100ng-35ug. But perhaps making your own tips might be cheaper.

Affinisep

During Masters thesis under Prof. Paul Haynes and Prof. Mark Molloy (Macquarie University) circa 2012-14, and a lot more as a technician at a core facility 2014-17 with @itsbinir.bsky.social hanging around.

Not sure, but we usually get >90% 0 missed cleavage with STrap and SP3 at 47C, 60 mins in 50mM TEAB/EPPS.

Congrats Tina!

Trying to find who is, and how. But I’m afraid many tribrids and QEs will need to be retired and replaced with TOFs if labs/core facilities are to keep up.

Any specific reason for OT-OT instead of OT-IT?

Haven’t tried DIA on lumos but I’m inclined to believe 2hrs/sample with FAIMS-OT-IT might actually be faster for the same quant ids.

Similar for us on ascend but for lumos which doesn’t support RTS, SPS-MS3 with 24 TMT18 fractions ends up being 2 days for about 8k+ quant. With large batches and IRS channel, the throughput feels very 2018(?).

‘30spd’ == anyone getting TMT16 or TMT32 fractions finished within a day with >8k proteins?