Category Archives: Protein expression profiles during sexual maturation in Geoduck

Protein expression profiles during sexual maturation in Geoduck

Bioanalyzer Data – Geoduck RNA from Histology Blocks

I received the Bioanalyzer data back for the geoduck foot RNA samples I submitted 20150422. The two samples were run on the RNA Pico chip assay.



Bioanalzyer 2100 Data File (XAD): SamWhite_Eukaryote Total RNA Pico_2015-04-23_13-04-16.xad

Data file requires 2100_Expert_B0208_SI648_SR2 version of the software (Windows).

Gel Representation




The samples look really good! As we’ve seen previously in shellfish RNA, there is a single, prominent rRNA band/peak with very little degradation (smearing and/or no prominent peak/band).

Will proceed with RNA isolation from the remaining histology blocks.


Bioanalyzer Submission – Geoduck Gonad RNA from Histology Blocks

Submitted 3μL (~75ng) of RNA from each of the two gonad samples isolated from foot tissue embedded in paraffin histology blocks 20150408 (to assess quality of RNA) to Jesse Tsai at University of Washington Department of Environmental and Occupational Health Science Functional Genomics Laboratory:

  • Geoduck Block 34
  • Geoduck Block 42

Jesse will determine if the samples should be run on the RNA Pico or the RNA Nano chips.


RNA Isolation – Geoduck Gonad in Paraffin Histology Blocks

Isolated RNA from geoduck gonad previously preserved with the PAXgene Tissue Fixative and Stabilizer and then embedded in paraffin blocks. See Grace’s notebook for full details on samples and preservation.


RNA was isolated from only two samples using the PAXgene Tissue RNA Kit (Qiagen) from the following geoduck sample blocks to test out the kit:

  • 34
  • 42


  • Prior to beginning, I prepared Buffer TR1 by adding 10μL of β-mercaptoethanol (β-ME) to 1000μL of Buffer TR1). This will be good for up to six weeks at RT.
  • Reconstituted DNase I with 550μL of RNase-free H2O. Aliquoted in 100μL volumes and stored @ -20C in the “-20C Kit Components” box.

Five 5μm sections were taken from each block.

Isolated RNA according to the PAXgene Tissue RNA Kit protocol with the following alterations:

  • “Max speed” spins were performed at 19,000g.
  • Tissue disruption was performed with the Disruptor Genie @ 45C for 15mins.
  • Shaking incubation step was performed with Disruptor Genie
  • Samples were eluted with 34μL of Buffer TR4, incubated @ 65C for 5mins, immediately placed on ice and quantified on the Roberts Lab NanoDrop1000.

Samples were stored at -80C in Shellfish RNA Box #5.

NOTE: The spreadsheet linked indicates other samples exist in the slots that I placed these two samples. Will need to update the spreadsheet to be accurate.




Looks like the kit worked! Yields are pretty good (~800ng) from each. The 260/280 ratios are great for both samples. Oddly, the 260/230 ratios for the two samples are pretty much polar opposites of each other; not sure why.

Will proceed with the remainder of the samples that were selected by Steven and Brent. Or, maybe I should try to make some cDNA from these RNA samples to verify the integrity of the RNA…