Monday, June 29, 2015

Summer Week 5

Week of June 22nd-25th

I haven't spent much time in lab this week. It was finals week for my math class and I needed to study. I did notice that a lot of my plates are beginning to grow some pretty lovely cultures. I now have at least 4 species of fungi growing in my plates but I am still unable to classify any of them.

I've been giving a lot of thought to where I want to take this project in the future. Depending on what I want to do my project can take me a lot of places. I could work with Cel and learn how to extract DNA and try to use that procedure on my endophytes. I could learn how to stain and identify the morphology of my fungal colonies. Or I could try and infect a different species with an endophyte and see if it changes the growth of the plant. Choices Choices


Thursday, June 25, 2015

Summer Week 4

Week of June 15th-18th

On the 3rd of June I found out that the method I was using to stain tissues to look for endophytes was not as effective as it could have been. By adding a drop of stain instead of excess alcohol when mounting my slide I am better able to see endophytic hyphae because the plant cells are not dehydrated from the alcohol. After altering my staining method I began to see more endophytes. I found three this week in silver leafed nightshade, mint and a succulent euphorbia plant.

The plates made last week began to grow endophytes and the ones from the week before continued to grow larger. The growth rate for all the colonies appears to be very slow which is a good sign they are genuine endophytes.

This week I also found a really neat new resource call the Journal of Video Experiments or JOVE. They have detailed videos of how to set up and conduct different experiments including the formulas used for the dilution of chemicals and things of that nature. One I watched was about how to inoculate plants with endophytes that kill insects. Here is the link, I don't know how to embed videos.

 http://www.jove.com/video/50360/establishing-fungal-entomopathogens-as-endophytes-towards-endophytic



Summer Week 3

The week of June 8th-11th

On Monday June 8th I decided to look at any of my Show Low specimens that looked fresh enough to still absorb dye under a microscope. I looked at six specimens and only one had anything that looked like an endophyte. A big problem I was having is seeing inside the leave of plants have have a low surface area such as pine needles and juniper. The shape of the leaves requires a lot of light pass through a dense area making things blurry and dark. It was also difficult to cut the leaves so I think I need to learn how to clear plant tissues using chemicals.

On the 8th I also noticed that one of my previous plates had some white fungal growth on it. The hyphae were clearly coming out of the interior of the leaf. There has been no evidence of contamination on any of the plates so I know my new sanitation method is working well.

I found another endophyte in a sample from a tree near D building, I'm not sure what the species is. As I was walking to the lab on Monday they were trimming the trees and I picked up a sample. I think it maybe some kind of African Acacia tree but I have no idea. The leaves were so covered in debris that it was difficult to see much inside the leaves. However in more than one place I found had what looked like fruiting bodies connected to hyphae most likely on the surface of the leaf instead of inside it. I plated some samples anyway.


Summer Week 2

The week of June 1-4 was spent processing the samples I collected from 40 acres of land just outside Show Low Jordan calls Tarantula Gardens.

I went to a few different sites on the land, chose a stand of juniper trees and marked off an area 35 feet around the trees using stakes. I collected samples from various plants inside the area and took notes and photos of the plants for later reference. I had intended to do three sites and collect some of the same species of plants at all the sites to see if there was a difference in endophytic colonization in the different areas. However, after building a fence all day I was so tired it didn't really work out that way. I collected ample samples from site number three and took a few samples of different species found at site two but then I was too bushed to continue and called it a day. I figured 24 samples was plenty to work with for awhile.

I made three major mistakes when I was collecting samples in Tarantula Gardens: 1. I didn't put each sample in its own individual bag but instead placed all samples of a certain size in one bag and all samples that were smaller in another bag. Despite noting in my lab book which bag I put each sample by the time I got back to the lab I couldn't tell any of the samples apart. This was especially true with the grass samples.
2. I didn't put a damp paper towel in the bags with the samples so by the time I was able to look at many of the plants they were dried out and brittle.
3. The photos I took of the plants were blurry, out of focus and did not include enough detail to identify any of the species. I need to be using a better camera meaning not my cell phone camera.


Tarantula Gardens Site #3:


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Summer Week 1

OK so I knew I needed to be blogging this summer, I've gotten several emails about it, but I couldn't find time with my math class. Summer classes move fast and I needed to spend as much time studying as possible. However, yesterday I had my final so now I have plenty of time to work on my blogs.

The last week of the Spring 2015 semester I made a pact with myself that I would take notes every single day that I was in the lab. I wont say that I've kept up with it 100% but I have been doing much better about keeping notes when in the lab. One day I will take beautiful, meticulous notes with ease.

I started the week by walking around campus and taking samples from some of the plants I found. I tried staining them with coomassie blue and rose bengal dye but was struggling with getting the dye to stick to the fungal mycelium and also with the rose bengal dye being too thick. I also didn't like the layout I chose for recording my notes and resolved to change it in the future.

On Thursday I went to Pinetop to visit and take more samples.

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