Grace’s Notebook: Thursday, December 14, 2017

(1) 2015 oyster seed data

I went through some more peptides on SkylineDaily with the 2015 oyster seed data. Protocol calls for checking ~100 peptides to ensure correct peak was selected (Step 5).

(2) Crab project

I met with Steven and Pam today to discuss the overall project and next steps.

Pam brought the most recent samples. There are three samples per crab, and 6 per warm-water treatment crabs (because only 3 survived). Total of 117 crabs.

I will save 50µl of hemolymph/RNAlater mixture for Pam from each crab (117 tubes total). Then I will spin down all the samples (114×3 + 3×6 = 360 samples total), remove and save the supernatant, and place supernatant and pellet tubes in -80.

In January, we will start processing the RNA and pooling the samples to be sent off for sequencing.


Yaamini’s Notebook: Remaining Analyses Part 13

Triple-nested for loops are not fun

As I mentioned in a previous post, Steven suggested I create a table with information about the peptide vs. biomarker regressions I did. I was trying to do that using a three for loops nested within eachother.

screen shot 2017-12-13 at 2 16 29 pm

It did not go well.

When I was talking with Sam today, he suggested I break the nested for loops. Instead, he thought I should save all of the regression information into a new table, and then reformat that information into the table I wanted to save. That was the right idea! The code can be found in this R Script, or below.

screen shot 2017-12-13 at 2 46 36 pm

screen shot 2017-12-13 at 2 46 51 pm

screen shot 2017-12-13 at 2 46 59 pm

The table I produced can be found here.

My next steps are to (finally) quality control my data, remake pH, DO and salinity plots, make a table of important environmental variables, and do something with the growth data. Oh, and write I guess.

…can you tell I’m a bit tired of this yet?


Grace’s Notebook: December 12, 2017

Crab hemolymph samples:

Pink-capped were sampled 11/10/2017

I spun down the hemolymph samples (5000g for 10min) and saved the supernatant and pellets in separate tubes. The boxes were placed in the -80 (tray 14).

Laura’s Notebook: December Goals (belated)

Time flies, especially when I get various waves of data that needs analyzing, and also Thanksgiving, tests/papers from class, etc… Lots of tasks will carry over from November, BUT nevertheless, headway has been made.

Olys at dock

  • Clean, measure broodstock (after hatchery meeting)

Geoduck proteomics

  • Finish Results section
    • Correlation btwn various parameters, protein abundance
    • Try to use Structural Equation Model instead of linear regression model
    • QA %>1SD & %>2SD calculations
  • Get more methods info from Micah, Emma
  • Focus on DISCUSSION
  • Identify target journals
  • Determine figures for paper. Candidates:
    • Box/violin plots of protein abundances by subbasin, including 3 peptides separately. Like this, but with 4 panes for each protein: img_3305
    • NMDS plot (like what I already have) with overlaying circles by subbasin
    • 3-pane plot of pH, T, and DO (continuous)? Would be messy with all 8 traces from each site.
    • Correlation matrices for: variables identified in model (DO var, pH >1sd %, and growth)
  • Remaining things that Emma said I should do:
    • Linear Response Plot, as per Emma: Peak area on the y, amount of peptide (moles) on the x. Don’t know absolute quantity of experimental peptides, could make the x-axis relative quantity or something. Can generate plots like these in MSstats.
    • DIA error rate
    • SRM dilution curve
  • Idea for paper, but would take a while (probably a few days): screen all proteins in DIA Skyline data for a “menu” of targetable, detectable proteins (based on visual check of chromatograms). This could be published alongside the paper as a very usable resource.
  • More lit Research
    • Growth related to protein expression – but why only some proteins were diff. expressed?
    • Bioassays
    • Determine if abundance difference is “biologically relevant.” If I can find SRM abundance good (haven’t found good references yet), OR find citable % diff.

Prep for Oly genetics hatchery vs. wild analysis

  • re-Read Fischer et al. 2012
  • Get most current data set from Crystal
  • ID best program to use

Application things

  • Finish NDSEG, get letters
  • AA travel awards (?)


  • Submit MS paperwork to office & proposal online (pending approval from Rick, Jackie)
  • Learn how to tag notebook posts
  • Create for proteomics data on Owl

In January:

  • Determine which Oly samples to sequence from last spring/winter
  • Meet with STATS resource to figure out how to analyze Oly larval survival – parse out survival data to 224um, to juvenile, by time for reps

On hold:

  • Record podcast pilot with Megan
  • Find local vendor that sells dry suits, try on to determine size, then purchase gear

Accomplishments from last month

  • Checked out Oly histology data from last year’s experiment
  • Cireculated MS proposal for approval from committee
  • Submitted NSA abstracts, travel grant app
  • Sampled experimental Olys for histology (time=0), got animals into treatments
  • Received collection permit @ Mud Bay, made contact with homeowners for access, collected first batch
  • Gave Oly shells to Heater @ Wood’s lab for Polydora inspection
  • Got the CoEnv travel grant for AA
  • Proteomics stuff:
    • Finalized SRM tech. rep filtering process
    • Tracked down tidal charts from each Geoduck Proteomics ouplant location; used to process/filter environmental data from Micah
    • Generated summary statstics on environmental data
    • Re-ran proteomics analyses on the peptide-level, where transitions within each peptide were summed. Lambda-transformed peptide abundance for normal distribution, then ran 2-way ANOVAs.
    • Learned how to run stepwise linear resgression models, ran on diff. expressed proteins with environmental summary stats.
    • Refined methods section of paper
    • Made headway on results section of paper
    • Drafted intro; will likely need to revise based on results
    • Finished parasite class things
    • Generated notebook for DIA data in Skyline
    • R-script for merging DIA results with annotations, extracting SRM targets from this dataframe
    • Generated peptide variability stats for paper
    • Discarded unecessary vials (the “just in case” vials, and autosampler vials prepped for mass spec). If I need to re-run samples, I’d prepare new autosamper vials from my digested peptides.

from LabNotebook

Grace’s Notebook: December 11, 2017

Crab Hemolymph Samples:

Green-capped were sampled 11/08/2017

I spun down the crab hemolymph samples and saved the supernatant and pellets in separate boxes. I spun them down at 5000g for 10 minutes. Then, I placed the boxes in the trays in the left -80. (Tray 8 and Tray 10)

I only got through the green-capped samples today.

Yaamini’s Notebook: Sequencing Protocol Thoughts

a.k.a. How to take a break from proteomics

Instead of poring over environmental data, I worked on an MBD-Sequencing protocol for the Crassostrea virginica gonad samples this week. Turns out I know absolutely nothing about different sequencing protocols, so I had to do a bunch of reading about bisulfite sequencing.

Here’s what I learned from a general literature review:

  • Most papers are focused on either plant, mice or human epigenomes. Those are not invertebrates.
  • According to Olova et al. 2017, “amplification-free and post-bisulfite procedures should become the gold standard for [Whole Genome Bisulfite Sequencing (WGBS)] library preparation”
  • MBD-Seq is not the same as WGBS! It’s called lots of things, like MethylCap-Seq. According to this Illumina post, proteins bind to methylated cytosines, then precipitated out using beads.
  • MeDip uses antibodies. Riviere et al. 2017 used this method to profile Pacific oyster methylomes at different methylation states, so it would probably work with C. virginica. However, bisulfite sequencing methods are found to be more accurate. We’re going to ignore this method.

After learning about the different sequencing methods, I reviewd the methods section from Gavery and Roberts 2013.

  • Sheared DNA was incubated with MBD-Biotin Protein and dynabeads following MethylMinder instructions
  • Enriched DNA was eluted from the beads and purified
  • Illumina Tru-Seq adapters were used to prepare the DNA libraries
  • Qiagen’s EpiTect Bisulfite Kit was used for bisulfite treatment
  • Library preparation and sequencing were done on the Illumina HiSeq 2000

This protocol matches with Olova et al. 2017’s suggestion of post-bisulfite treatment and no PCR amplification. However, I don’t know much about the kits she used, and whether or not there are better alternatives. Kurdyukov and Bullock 2016 lay out information for MethylCap (Diagenode) and MethylMiner, but don’t really compare the efficacy of the two. I’m going to ping Sam and Mac to see if they have any opinions on the kits.

My overall takeway is that Mac’s protocol should be sufficient for our work!


Yaamini’s Notebook: December Goals


(Now I have November and December Dwights!)

So…I guess it’s the end of the year now. Welp. Cue the cramming of work into what’s left of the quarter!

November Goals Recap:

  • Turned in my milestone paperwork!
  • Successfully presented at GSS and WSN
  • Half-completed my DNR Proteomics paper
    • Revised methods and results
    • Outlined discussion
    • Made good progerss on integrating many data sources for my analyses

December Goals:

  • Finish. this. proteomics. paper.
  • Identify sequencing protocol for C. virginica gonad samples
  • Prepare C. virgincia samples for sequencing
  • Add Disqus to my blog