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The Crinoid Project:Genetic bar-coding of a cryptic species?
By: Olivia Storrs
What is a Crinoid?• Marine animals inphylum Echinodermata
• Common as fossils – typically stalked
• Davidaster rubiginosa, Davidaster discoidea –Comatulidae – extant stalklesscrinoids
• These species may be found on shallow reefs
Objective
• To test, through genetic bar-coding, the hypothesis that a cryptic species of crinoid exists within Davidaster.
• Why is this important? – Identifying full genetic diversity allows better understanding of fragile tropical reef ecosystems.
Davidaster discoidea
Davidaster rubiginosa
???? Cryptic intermediate ????
Methods• 1: Obtain sample• 2: Extract DNA• 3: Clean/Prep DNA• 4: Perform PCR reactions• 5: Run gels• 6: If PRC successful, prep for sequencer• 7: Complete PCR reaction• 8: Sequence• 9: Create new primers with sequence • 10: Analysis
Collecting Samples
Sample acquisition led us to San Salvador, Bahamas where we could find two of the three crinoids in question right off the coast.
Lab Work
This particular crinoid (D. discoidea) was extracted from a reef, brought to the research facility for observation in a water table, and inspected under a microscope. The next day it was returned to its reef with no harm done.
D. discoideaPartial arms were collected
D. discoidea oral disc under a microscope with food transporting pinnules
Once all samples were collected, the extraction process commenced.
Beginning Extractions
Labeling and creating individual samples
Labeled samples
Extraction –cleaning and buffering
Back at Home – Cincinnati Museum Center Molecular Genetics Lab
Immediately upon return from the Bahamas, Polymerase Chain Reactions (PCR) began. After several unsuccessful attempts to amplify the DNA, it was decided that another round of extractions should be done in the comfort of our own lab.
Polymerase Chain Reaction- Amplifying DNA
• Literature search to find Primers
• Record list of Primers for purchase
• Order
• Wait/Receive
• Set up PCR
Performing PCR
• Requires exact measurements of
– Water
– Taq (thermostableT. aquaticus
DNA polymerase)
– Forward and reverse primers
– DNA
A Graph Illustrating PCR
www.mun.ca
After PCR, one must check to see if amplification was successful by
inserting PCR’d sample and loading dye into a Gel
Electrophoresis apparatus.
Gel is ‘run’ and then placed over ultraviolet light. This is an example of
what you should see.
Sequencing
• Used PRC’d sample for sequencing prep
• Ran a different program in PCR machine to complete sequencing reaction
• Once sequenced, collected sample sequence was used to create new primers for increased precision in amplification results
• Amplified DNA with crinoid-specific primers
The catch…
•Preliminary sequences are not adequate –sampled tissues did not yield full genetic code
Originally, to spare crinoids, we only sampled their arms (able to regenerate). Unfortunately, DNA amplification has led to mixed results. There appears to be little tissue in crinoid arms and we may need to collect larger crinoid samples for better results.
What’s Next?
• Obtain better samples (Jamaican expedition planned)
• Repeat amplification process
• Sequence and read genetic code
• Compare with knownDavidastercrinoids
• Test hypothesis of cryptic species
Thank You!
I would like to give a big thank you to the Cincinnati Museum Center, The National Geographic Society for travel funds, Professor David Meyer, his wife
Kani, Dr. Herman Mays, and my father.