{"id":544,"date":"2016-07-05T08:52:30","date_gmt":"2016-07-05T14:52:30","guid":{"rendered":"http:\/\/ciresblogs.colorado.edu\/reccs\/?p=544"},"modified":"2016-07-05T08:52:30","modified_gmt":"2016-07-05T14:52:30","slug":"making-serious-mistakes","status":"publish","type":"post","link":"https:\/\/ciresblogs.colorado.edu\/reccs\/2016\/07\/05\/making-serious-mistakes\/","title":{"rendered":"Making Serious Mistakes"},"content":{"rendered":"<p><a href=\"http:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/CYC-NF-NSP1-2.jpg\"><img loading=\"lazy\" decoding=\"async\" class=\"size-medium wp-image-545 alignleft\" src=\"http:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/CYC-NF-NSP1-2-300x169.jpg\" alt=\"CYC-NF-NSP1 (2)\" width=\"300\" height=\"169\" srcset=\"https:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/CYC-NF-NSP1-2-300x169.jpg 300w, https:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/CYC-NF-NSP1-2-768x432.jpg 768w, https:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/CYC-NF-NSP1-2-1024x576.jpg 1024w, https:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/CYC-NF-NSP1-2-640x360.jpg 640w\" sizes=\"auto, (max-width: 300px) 100vw, 300px\" \/><\/a>This week I scraped all of soil bacteria off of the agar plates, extracted DNA from the samples, prepped and put the gDNA samples through PCR, checked the PCR results using gel electrophoresis, put another set of gDNA samples through another round of PCR, combined all of the resulting amplicons and prepped them for sequencing, took the samples to a sequencing center to be sequenced, prepped a mapping file on Excel, met with Jennifer to discuss my project and this upcoming week\u2019s newsletter, and did some Rstudio training. In the communication workshop, I learned what effective figures look like and how to write and present the results section of a scientific paper.<\/p>\n<p>This week I made a major mistake. After scraping a bacteria sample off of the agar plate it was cultivated on, an<a href=\"http:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/Plate-Scraping-2.jpg\"><img loading=\"lazy\" decoding=\"async\" class=\"size-medium wp-image-546 alignright\" src=\"http:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/Plate-Scraping-2-300x169.jpg\" alt=\"Plate Scraping 2\" width=\"300\" height=\"169\" srcset=\"https:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/Plate-Scraping-2-300x169.jpg 300w, https:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/Plate-Scraping-2-768x432.jpg 768w, https:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/Plate-Scraping-2-1024x576.jpg 1024w, https:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/Plate-Scraping-2-640x360.jpg 640w\" sizes=\"auto, (max-width: 300px) 100vw, 300px\" \/><\/a> applicator that looks a lot like a large Q-tip is used to absorb all of the bacteria into a cotton tip which is then cleaved off and placed in a 2 mL tube. This tube is then used in the first step of DNA extraction. DNA extraction consists of several steps \u2013 bursting the cells open to get their DNA into solution and then successive steps are used to isolate the DNA from all other organic and nonorganic substances. Each step requires a new 2 mL tube, resulting in 6 total tubes per sample. The last tube will have the isolated DNA. It\u2019s important when performing this procedure to label the last tube (the 6<sup>th<\/sup> one) really well since this is where the DNA will be stored.<\/p>\n<p><a href=\"http:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/All-DNA-Extractions.jpg\"><img loading=\"lazy\" decoding=\"async\" class=\"size-medium wp-image-547 alignleft\" src=\"http:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/All-DNA-Extractions-300x169.jpg\" alt=\"All DNA Extractions\" width=\"300\" height=\"169\" srcset=\"https:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/All-DNA-Extractions-300x169.jpg 300w, https:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/All-DNA-Extractions-768x432.jpg 768w, https:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/All-DNA-Extractions-1024x576.jpg 1024w, https:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/All-DNA-Extractions-640x360.jpg 640w\" sizes=\"auto, (max-width: 300px) 100vw, 300px\" \/><\/a>In previous extractions I would simply just number the tubes for each sample and include a key in my lab notebook to differentiate them. I noticed that the DNA extractions that Tess performed were labelled differently and in such a way that it was easier to identify them faster. For example, for a tube containing north-facing slope soil bacteria that did not undergo the ethanol treatment and was cultivated on an agar plate with the addition of peptidoglycan fragments &#8211; she labelled it as \u201cP-NF-NSP1\u201d. \u201cP\u201d stood for \u201cpeptidoglycan\u201d, \u201cNF\u201d stood for \u201cnorth-facing slope\u201d, \u201cNSP\u201d stood for \u201cnot spore selected\u201d, and \u201c1\u201d indicated which replicate the sample came from (was labelled 1, 2, or 3). In an attempt to be better about labelling, I decided to model myself <a href=\"http:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/DNA-Extraction.jpg\"><img loading=\"lazy\" decoding=\"async\" class=\"size-medium wp-image-548 alignright\" src=\"http:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/DNA-Extraction-300x169.jpg\" alt=\"DNA Extraction\" width=\"300\" height=\"169\" srcset=\"https:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/DNA-Extraction-300x169.jpg 300w, https:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/DNA-Extraction-768x432.jpg 768w, https:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/DNA-Extraction-1024x576.jpg 1024w, https:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/DNA-Extraction-640x360.jpg 640w\" sizes=\"auto, (max-width: 300px) 100vw, 300px\" \/><\/a>after her. I labelled the last tubes in my extraction as \u201cCY-NF\u201d or \u201cCY-SF\u201d to indicate \u201ccyclic AMP\u201d and \u201cnorth-facing slope\u201d or \u201csouth-facing slope\u201d. I did not, however, include whether or not these samples had undergone ethanol treatment (\u201cSP\u201d) or not (\u201cNSP). I didn\u2019t realize that this would be a problem until I was on the very last step of the extractions and placed the last tubes with these labels into the centrifuge. There were 6 samples with the label \u201cCY-NF\u201d and 6 with the label \u201cCY-SF\u201d. My heart sank once I realized that there was no way for me to differentiate which half of these samples had undergone the ethanol treatment and which ones hadn\u2019t. I began to panic realizing that there was no way to turn back. The sequencing run was scheduled later in the week and there was no time to make new agar plates, incubate the bacteria again, and to perform the extractions again.<\/p>\n<p>I immediately told Tess what happened and she was incredibly understanding. She told me to take this mistake as a lesson in the importance of labeling as specifically as possible. The good news was that visibly when observing the agar plates, there were noticeable colony differences between plates with soil bacteria that had undergone the ethanol treatments in comparison to those that hadn\u2019t. More than likely the sequencing results will show differences in microbial composition between the two conditions. This definitely gave me some peace of mind. We will not, however, be able to determine which replicate number the samples were. I tried my best not to be too hard on myself for making a mistake that was entirely preventable.<\/p>\n<p>I definitely learned that it\u2019s important not to get too wrapped up in the procedure of an experiment and to understand fully what\u2019s happening conceptually. I had completed the first round of PCR for all of the soil bacteria DNA extractions and performed gel electrophoresis to verify the presence of amplicons for each sample. Every other occasion that I had completed gel electrophoresis, Tess took the PCR tray with all of the amplicons and stored them somewhere \u2013 a step in our experimental procedure that I hadn\u2019t discussed with her or seen. After I had finished the gel electrophoresis, I messaged her on my computer to ask her if it was OK for me to toss the PCR plate I had made. My rational behind this question was that we had a separate tray in a freezer that contained all of the DNA extractions already. Tess came into the lab and told me that we should definitely NOT throw the PCR plate because the amplicons were what would be used to sequence, not the DNA from the extraction tray. I felt stupid for a moment, realizing that there was a major gap in my understanding of the procedure. Thankfully, I didn\u2019t toss the PCR products without asking, so this misunderstanding didn\u2019t result in any problems with the experiment \u2013 but I realize how I could have answered this question myself if I had simply thought about what the PCR tray represented conceptually. I was mixing up two different terms: gDNA, which is simply the DNA extracted from the bacterial samples, and amplicons, which are copies of a specific gene from all the samples that results from performing PCR on the gDNA. I give myself some credit for being abruptly placed in a professional setting with a plethora of terminology I haven\u2019t ever used before and still managing to catch on relatively quickly to the experimental procedure, but I certainly know now that I need to slow down and really make sure that I understand what every component in the experiment is and what is happening at each step of the procedure.<\/p>\n<p><a href=\"http:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/Amplicon-Solution-Final-Product.jpg\"><img loading=\"lazy\" decoding=\"async\" class=\"size-medium wp-image-549 alignleft\" src=\"http:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/Amplicon-Solution-Final-Product-300x169.jpg\" alt=\"Amplicon Solution Final Product\" width=\"300\" height=\"169\" srcset=\"https:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/Amplicon-Solution-Final-Product-300x169.jpg 300w, https:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/Amplicon-Solution-Final-Product-768x432.jpg 768w, https:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/Amplicon-Solution-Final-Product-1024x576.jpg 1024w, https:\/\/ciresblogs.colorado.edu\/reccs\/wp-content\/uploads\/sites\/46\/2016\/07\/Amplicon-Solution-Final-Product-640x360.jpg 640w\" sizes=\"auto, (max-width: 300px) 100vw, 300px\" \/><\/a>To be honest, this week was a rough one for me. There was a lot of pressure to get everything prepared in time for the sequencing run on Thursday which required me to do laboratory techniques that I\u2019d only performed once or a few times the week prior. I\u2019m unquestionably proud of myself for pulling through this week and maintaining my cool in the midst of some major mistakes. It\u2019s easy to get down on myself when I don\u2019t perform everything to the standard that I expect of myself, but I cherish these moments for the belief that they\u2019ll solidify my ability to persevere through unexpected adversity. I\u2019m happy that I\u2019m determining each day the reality that is the challenge of being a research scientist. My powerful desire to perform my experimental procedure as accurately and error-free as possible proves to me how strongly I strive to obtain results that are true to my research question. I didn\u2019t realize just how important this project was to me until I started making some major mistakes that could seriously compromise the results. I\u2019ve truly internalized this project as something of great value for my own personal growth and to the field of microbial ecology.<\/p>\n","protected":false},"excerpt":{"rendered":"<p>This week I scraped all of soil bacteria off of the agar plates, extracted DNA from the samples, prepped and put the gDNA samples through PCR, checked the PCR results using gel electrophoresis, put another set of gDNA samples through another round of PCR, combined all of the resulting amplicons and prepped them for sequencing,&hellip; <a class=\"read-more\" href=\"https:\/\/ciresblogs.colorado.edu\/reccs\/2016\/07\/05\/making-serious-mistakes\/\">Read More<\/a><\/p>\n","protected":false},"author":79,"featured_media":0,"comment_status":"open","ping_status":"open","sticky":false,"template":"","format":"standard","meta":{"footnotes":""},"categories":[4],"tags":[],"class_list":["post-544","post","type-post","status-publish","format-standard","hentry","category-reccs-2016"],"jetpack_featured_media_url":"","publishpress_future_action":{"enabled":false,"date":"2026-07-23 22:12:01","action":"change-status","newStatus":"draft","terms":[],"taxonomy":"category"},"publishpress_future_workflow_manual_trigger":{"enabledWorkflows":[]},"_links":{"self":[{"href":"https:\/\/ciresblogs.colorado.edu\/reccs\/wp-json\/wp\/v2\/posts\/544","targetHints":{"allow":["GET"]}}],"collection":[{"href":"https:\/\/ciresblogs.colorado.edu\/reccs\/wp-json\/wp\/v2\/posts"}],"about":[{"href":"https:\/\/ciresblogs.colorado.edu\/reccs\/wp-json\/wp\/v2\/types\/post"}],"author":[{"embeddable":true,"href":"https:\/\/ciresblogs.colorado.edu\/reccs\/wp-json\/wp\/v2\/users\/79"}],"replies":[{"embeddable":true,"href":"https:\/\/ciresblogs.colorado.edu\/reccs\/wp-json\/wp\/v2\/comments?post=544"}],"version-history":[{"count":5,"href":"https:\/\/ciresblogs.colorado.edu\/reccs\/wp-json\/wp\/v2\/posts\/544\/revisions"}],"predecessor-version":[{"id":555,"href":"https:\/\/ciresblogs.colorado.edu\/reccs\/wp-json\/wp\/v2\/posts\/544\/revisions\/555"}],"wp:attachment":[{"href":"https:\/\/ciresblogs.colorado.edu\/reccs\/wp-json\/wp\/v2\/media?parent=544"}],"wp:term":[{"taxonomy":"category","embeddable":true,"href":"https:\/\/ciresblogs.colorado.edu\/reccs\/wp-json\/wp\/v2\/categories?post=544"},{"taxonomy":"post_tag","embeddable":true,"href":"https:\/\/ciresblogs.colorado.edu\/reccs\/wp-json\/wp\/v2\/tags?post=544"}],"curies":[{"name":"wp","href":"https:\/\/api.w.org\/{rel}","templated":true}]}}