Skip to main content

Sarah- Week 4

Going into this week, I was a little bit terrified.  My grad student, being away this week, had left me a list of tasks to complete and some protocols.  I really did not want to have to send a text to her saying, "Please help.  I messed up a lot!"  (spoiler alert: I didn't have to) My first job on Monday was to rinse a primary antibody off of western blots and to then put on a secondary.  I was in charge of four westerns which had different lid covers and were all slightly different from each other.  Two westerns followed one protocol and the other two followed another protocol.  When I put the westerns down, I oriented them in a certain way so that I would not accidentally switch the lids.  I then had to rinse off the secondary and expose the westerns to ECL in order for the proteins to become visible in the imager.  After successfully imaging the westerns, I used the stripping buffer in order to prepare them for the next primary, in order to repeat the process again the next day.  I very carefully walked the western blots over to the cold room to allow them to incubate overnight on the rocker.
Next, I had to fix two plates of cells and then do the first day of the cell-staining procedure.  The cells were first sitting in media which had a salmon pink color to it.  I had to first vacuum out this media and then rinse the cells with PBS and PBSt solution.  It was really important not to confuse PBS with PBSt because PBSt contains a detergent which is not in PBS.  I also had to treat the plates with Cy3 or FitC depending on the step.  I have found that a lot of research is waiting time, which felt a little longer than usual this week with a few less people in the lab than usual due to the 4th of July.
The next day, I repeated the western procedure and reimaged the blots before beginning the second day of the cell- staining procedure.  As the plates were now light sensitive, I had to keep them wrapped in tin foil.  I have gotten into the habit of leaving them in a drawer by the vacuum when they are not on a rocker in order to keep them out of the way and out of the light.  After all of the westerns and the plates were placed on the rocker in the cold room, I extracted DNA from tail samples in order to prepare them for PCR.  There were only two samples, but the controls, including no DNA, also had to be put into the PCR machine.
On Wednesday and Thursday, I was able to spend time with my cousin and parents, thanks to 4th of July.
On Friday, I was back in the lab!  I added loading dye to my PCR-ed samples before running them in a gel for an hour.  During this time, I began the western procedure once again, and continued with day 3 of the cell staining procedure.  While the cell plates were incubating, and the westerns were resting on the rocker, I imaged the gel.  The image was a little bit streakier than I would have liked, probably due to an excess of DNA being loaded, but I was overall happy with my work.
I was really proud of myself this week for being able to manage a few different things, finding all the necessary chemicals, and for going through the procedures without becoming confused by all of the steps.

Comments

  1. Sounds like you did a great job keeping it all organized!

    ReplyDelete

Post a Comment

Popular posts from this blog

Evan Bradley, Week 3 at the Missouri Orthopaedic Institute

As mentioned in my previous blog, I have been awaiting ligament, menisci, and cartilage tissue from a canine or human knee joint for (interleukin) IL-1B tissue culture. IL-1B is an inflammatory cytokine that has been proven to increase rates of tissue degeneration and osteoarthritis development in the Thompson Lab. Dr. Stoker wants me to experiment with different types of knee tissues in a co-culture with varying levels of this cytokine to determine its effects on the entire knee joint. This co-culture uses an insert permeable to the media to separate the two tissue samples from physical contact, while allowing them to share the same media. This creates an extremely accurate model for knee tissues in their native environment due to their exposure to the same synovial fluid in the joint. This model would then be treated with the IL-1B and cultured for 21 days. During these 21 days, the media would be collected every three days for biomarker evaluation at the end of the stu...

Kylie Heering, Week 2 at the Goldstein Lab

We started off our week with a congratulatory acai bowl trip to celebrate Preston’s acceptance into a training grant program. Acai bowls in California top Playa Bowls (no question about it). From what I can tell, its a pretty huge honor to be recognized by this grant, but he’s really humble about it. On Monday, Preston and I decided that testing antibodies that have never been tested on prostate epithelial cells before would be a good objective for my first Western blot on my own. We needed to probe for ASCT2, a glutamine transporter, and GLS in order to determine if their corresponding antibodies are functional. Antibodies are crucial for Western blots because they bind to the protein of interest (POI), allowing for us to qualify its expression after imaging. As such, Preston wanted to make sure they worked by probing for ASCT2 and GLS on three different cell lines. Cell lines are commercially purchased human cells that have been immortalized (modified to grow indefinitely) by telome...

Daniel Cheng, In My Own Room

I had no idea that Pennsylvania is this wide. Within the first hour, my train had reached Philly. But to Pittsburgh, it took another seven. Even before I stepped foot into the Search-Based Planning Lab, I was waylaid by some anxious news. The PhD student assigned to be my mentor, Dhruv, texted me that he, Dr. Likhachev, and most of the lab would be out of town for the entire week. So that was that. Fortunately, it was my first week, the week to be spent learning new material, and Dhruv provided me with plenty to digest. I already had ROS (Robot Operating System) installed, so I looked towards the tutorials that ROS provided. I copied commands into my Linux laptop's terminal to run ROS features. I learned the basic structure of ROS: packages, services and clients, publishers and subscribers, messages, nodes, and topics (which nodes communicate messages over). There was one simple yet interesting program I came across in the tutorials called turtlesim, for which using only 2 comm...