Team:Yale/Interlab
From 2014.igem.org
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<strong>Section I: Provenance and Release <br> | <strong>Section I: Provenance and Release <br> | ||
- | 1 | + | <ol type="1"> <li>Who did the actual work to acquire these measurements? <br> </strong> |
The Interlab measurement study was conducted by Ariel Leyva-Hernandez, Yamini Naidu, and Stephanie Mao. <br> | The Interlab measurement study was conducted by Ariel Leyva-Hernandez, Yamini Naidu, and Stephanie Mao. <br> | ||
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- | + | <li> What other people should be credited for these measurements? (i.e., who would be an author on any resulting publication. For example, your faculty advisor may have helped design the protocols that you ran.) <br> </strong> | |
The study was conducted in Dr. Farren Isaacs’s lab, with the mentoring of Natalie Ma. <br><strong> | The study was conducted in Dr. Farren Isaacs’s lab, with the mentoring of Natalie Ma. <br><strong> | ||
- | + | <li> On what dates were the protocols run and the measurements taken? (this will often be a range of dates; make sure you say which data was taken at what times.) <br> </strong> | |
The construct protocols were finalized at the end of June, and the constructs were made over the span of July 21-September 3. The measurements were taken on September 9, 2014, and again on September 12, 2014. <br> | The construct protocols were finalized at the end of June, and the constructs were made over the span of July 21-September 3. The measurements were taken on September 9, 2014, and again on September 12, 2014. <br> | ||
<strong> | <strong> | ||
- | + | <li> Do all persons involved consent to the inclusion of this data in publications derived from the iGEM interlab study? <br></strong> | |
All persons mentioned give consent for their names to be included in the study. <br> | All persons mentioned give consent for their names to be included in the study. <br> | ||
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- | What is the model and manufacturer? How is it configured for your measurements? (e.g., light filters, illumination, amplification) <br></strong> | + | <li>What is the model and manufacturer? How is it configured for your measurements? (e.g., light filters, illumination, amplification) <br></strong> |
- | A Synergy H1 Plate Reader (BioTek, Winooski, VT) was used for all optical measurements. The instrument uses a Xenon flash lamp as a light source. Fluorescence measurements were taken at single wavelengths ( λex = 485 ± 4 nm and λem = 528 ± 4 nm). A bottom fluorescence measurement was taken, which is configured with double grating monochromators. The reading speed for fluorescence and absorbance measurements for a 96-well plate is 11 seconds. Two photomultiplier tubes are used for detection: one for the monochromator system and another for the filter system. <br><br><br> | + | A Synergy H1 Plate Reader (BioTek, Winooski, VT) was used for all optical measurements. The instrument uses a Xenon flash lamp as a light source. Fluorescence measurements were taken at single wavelengths ( λex = 485 ± 4 nm and λem = 528 ± 4 nm). A bottom fluorescence measurement was taken, which is configured with double grating monochromators. The reading speed for fluorescence and absorbance measurements for a 96-well plate is 11 seconds. Two photomultiplier tubes are used for detection: one for the monochromator system and another for the filter system. <br><br><br> </ol> |
Revision as of 00:11, 17 October 2014
Interlab |
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Section I: Provenance and Release
Fluorescence readings that diverged from the other samples of the same type by more than 50% were excluded from the data set; however, no such issues were encountered. 5. What exactly were the controls that you used? During the growth phase of the cell cultures, the ancestral DH5α strain was also grown in LBmin and subject to the same antibiotic selection marker: kanamycin or chloramphenicol. Clear cultures after a day of incubation signified selection for the retention of the target plasmids. All cultures were seeded at the same time and allowed to grow for the same duration. 6. What quantities were measured? (e.g., red fluorescence, green fluorescence, optical density) Green fluorescence and optical density were measured. 7. How much time did it take to acquire each set of measurements? A time lapse of about five minutes occurred between each data set. The plates were seeded and incubated for 12 hours prior to measurement. 8. How much does it cost to acquire a set of measurements? We are only considering the cost of the non-renewable materials, which were consumed during our measurements. Below is a chart of the resources used: Reagent/Material Cost Gibson Assembly mix $31.40 LB and LB Plate $5.00 96 well plate $2.00 Total $38.40 9. What are the practical limits on the number or rate of measurements taken with this instrument and protocol? The DH5α strain used was not a robust strain, and its growing time greatly impeded construct creation and measurement. Section III: Measured Quantities 1. For each type of quantity measured (e.g., fluorescence, optical density), report on the following: 2. Units: What are the units of the measurement? Fluorescence was measured in relative fluorescence units (RFU). Optical Density was measured in absorbance units (AU). What is the equivalent unit expressed as a combination of the seven SI base units? (http://en.wikipedia.org/wiki/SI_base_unit) . Absorbance in AU is a ratio, and thus has no SI units. i. RFU is an arbitrary fluorescence unit and cannot be compared. 3. Precision: What is the range of possible measured values for this quantity, using your instrument as configured for these measurements? (e.g., a meter stick measures in the range of 0 to 1 meter) i. Dynamic range: 0-4 OD What are the significant figures for these measurement? (e.g., on a meter stick, it is common to measure to the nearest millimeter). i. 0.0001 OD Is the precision the same across the entire range? If not, how does it differ? i. Yes How did you determine these answers? i. Synergy H1 Specification Sheet 2. Accuracy: When was the instrument last calibrated? . March 2013 How was the instrument calibrated? . An accredited BioTek technician calibrated the machine against a known standard concentration gradient during initial setup of the machine. Section IV: Measurements 1. For each sample, report: the identity of the sample each quantity directly measured each quantity derived from measurements (e.g., fluorescence/OD) |