Difference between revisions of "Team:NUDT CHINA/InterLab"
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<h3 style="font-size: 28px;margin-bottom: 10px;margin-top: 15px;">2. Preparation</h3> | <h3 style="font-size: 28px;margin-bottom: 10px;margin-top: 15px;">2. Preparation</h3> | ||
<p alt="content_add" style="font-size: 18px;">To start with, our team transformed E.coli strain DH5α with the provided plasmids, namely Test Device 1,2,3,4,5,6, Positive Control, and Negative Control. As long as colonies had emerged on Cm+ Resistance Media, we picked up 2 colonies in each petrie dish and cultured them at 37℃ with 220 rpm frequency for 14 hours. When the bacteria solutions were turbid enough, we began the following process. | <p alt="content_add" style="font-size: 18px;">To start with, our team transformed E.coli strain DH5α with the provided plasmids, namely Test Device 1,2,3,4,5,6, Positive Control, and Negative Control. As long as colonies had emerged on Cm+ Resistance Media, we picked up 2 colonies in each petrie dish and cultured them at 37℃ with 220 rpm frequency for 14 hours. When the bacteria solutions were turbid enough, we began the following process. | ||
| + | </p> | ||
| + | <h3 style="font-size: 28px;margin-bottom: 10px;margin-top: 15px;">3. OD600 Reference Point</h3> | ||
| + | <p alt="content_add" style="font-size: 18px;">With plate reader, we measured Abs600 of the LUDOX and H2O. The H2O measurement served as the background. Both included 4 technical replicates to enhance the reliability of the results. Comparing to the standard OD600 reference given, which was 0.0425, we were able to achieve a ratio between OD600 and Abs600. The ratio was essential in converting Abs600 raw measurements into standard OD600 records. | ||
| + | </p> | ||
| + | <h3 style="font-size: 28px;margin-bottom: 10px;margin-top: 15px;">4. Fluorescein Standard Curve</h3> | ||
| + | <p alt="content_add" style="font-size: 18px;">Different concentrations of fluorescein were obtained by 2-fold serial dilution. In the first pipet, 200μL Fluorescein 1×stock solution was added. By removing half of the 200μL solution in previous pipets to later ones which already contained 100μL PBS, we were able to generate 11 solutions in half-descending fluorescence concentration. We also included another pipet with 100μL PBS only as blank. Within each concentration, we performed 4 replicates to calculate the more representative mean. After the results were recorded, all fluorescein concentrations were divided by average fluorescence measurement, of which the medium-high mean were calculated to diminish operation errors. This mean point would be used to set up the conversion between fluorescein concentration and fluorescence measurements in later steps. | ||
| + | </p> | ||
| + | <h3 style="font-size: 28px;margin-bottom: 10px;margin-top: 15px;">5. OD600 and Fluorescence Measurements</h3> | ||
| + | <p alt="content_add" style="font-size: 18px;">We tracked the original OD600 of the 16 samples so as to dilute them into 0.02. Once the original values were available, we integrated them into the dilution calculation sheet and followed the suggested volume to dilute each sample. After dilution, we confirmed that OD600 had reached exactly 0.02 or around. Our team set that time as T=0(h) and measured average OD600 from 4 replicates of each 16 samples to reduce technical error. Other 4 replicates were used for T=0(h) fluorescence measurements, with the same equipment and settings in Step 3. Henceforward, we recorded the OD600 and fluorescence when T=0 and T=6. | ||
| + | </p> | ||
| + | <h3 style="font-size: 28px;margin-bottom: 10px;margin-top: 15px;">6. Equipments and Settings</h3> | ||
| + | <p alt="content_add" style="font-size: 18px;">To obtain OD600 measurement, we employed Multiscan FC. Single wavelength of 600nm was used, and path length correction was turned off. To reduce measurement error, we also added a dynamic circulation of 5 times, with 2-second intervals. | ||
| + | </p> | ||
| + | <p alt="content_add" style="font-size: 18px;">The fluorescence measurement was obtained through Fluoroskan Ascent FL and Thermo Fisher. The filters used were 485nm and 538nm for excitation and emission respectively. The measurement cycled 5 times with intervals of 2 second. | ||
</p> | </p> | ||
</div> | </div> | ||
Revision as of 09:40, 10 August 2018
Development of A Novel
Blood-MicroRNA Handy Detection System with CRISPR
InterLab
Introduction
The InterLab this year has been updated to a more detailed protocol. During the InterLab study, we used the LUDOX, fluorescence and the plasmids that were shipped along with the distribution kit, and closely followed the InterLab study protocol.
Through the InterLab 2018 study, we experienced a lot in the measuring work, and surprisingly got to know more about the instruments that usually were ignored by us. Actually, it is the measuring instruments that help us complete the project every year!!
Methods and Design
1. InterLab Parts
Positive Control (BBa_I20270)
NegativeControl (BBa_R0040)
Test Device1 (BBa_J364000)
Test Device2 (BBa_J364001)
Test Device3 (BBa_J364002)
Test Device4 (BBa_J364007)
Test Device5 (BBa_J364008)
Test Device6 (BBa_J364009)
2. Preparation
To start with, our team transformed E.coli strain DH5α with the provided plasmids, namely Test Device 1,2,3,4,5,6, Positive Control, and Negative Control. As long as colonies had emerged on Cm+ Resistance Media, we picked up 2 colonies in each petrie dish and cultured them at 37℃ with 220 rpm frequency for 14 hours. When the bacteria solutions were turbid enough, we began the following process.
3. OD600 Reference Point
With plate reader, we measured Abs600 of the LUDOX and H2O. The H2O measurement served as the background. Both included 4 technical replicates to enhance the reliability of the results. Comparing to the standard OD600 reference given, which was 0.0425, we were able to achieve a ratio between OD600 and Abs600. The ratio was essential in converting Abs600 raw measurements into standard OD600 records.
4. Fluorescein Standard Curve
Different concentrations of fluorescein were obtained by 2-fold serial dilution. In the first pipet, 200μL Fluorescein 1×stock solution was added. By removing half of the 200μL solution in previous pipets to later ones which already contained 100μL PBS, we were able to generate 11 solutions in half-descending fluorescence concentration. We also included another pipet with 100μL PBS only as blank. Within each concentration, we performed 4 replicates to calculate the more representative mean. After the results were recorded, all fluorescein concentrations were divided by average fluorescence measurement, of which the medium-high mean were calculated to diminish operation errors. This mean point would be used to set up the conversion between fluorescein concentration and fluorescence measurements in later steps.
5. OD600 and Fluorescence Measurements
We tracked the original OD600 of the 16 samples so as to dilute them into 0.02. Once the original values were available, we integrated them into the dilution calculation sheet and followed the suggested volume to dilute each sample. After dilution, we confirmed that OD600 had reached exactly 0.02 or around. Our team set that time as T=0(h) and measured average OD600 from 4 replicates of each 16 samples to reduce technical error. Other 4 replicates were used for T=0(h) fluorescence measurements, with the same equipment and settings in Step 3. Henceforward, we recorded the OD600 and fluorescence when T=0 and T=6.
6. Equipments and Settings
To obtain OD600 measurement, we employed Multiscan FC. Single wavelength of 600nm was used, and path length correction was turned off. To reduce measurement error, we also added a dynamic circulation of 5 times, with 2-second intervals.
The fluorescence measurement was obtained through Fluoroskan Ascent FL and Thermo Fisher. The filters used were 485nm and 538nm for excitation and emission respectively. The measurement cycled 5 times with intervals of 2 second.
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| name | city | |
|---|---|---|
| Tanmay | Bangalore | 560001 |
| Sachin | Mumbai | 400003 |
| Uma | Pune | 411027 |
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