Latest revision as of 04:04, 14 October 2018

Applet Human Practices Experiment Project Team Awards

InterLab Study

"Measurement is fundamentally an act of communication." - Jacob Beal

Reliable and repeatable measurement is a key component to all engineering disciplines. The same holds true for synthetic biology, which has also been called engineering biology. However, the ability to repeat measurements in different labs has been difficult. The Measurement Committee, through the InterLab study, has been developing a robust measurement procedure for green fluorescent protein (GFP) over the last several years. We chose GFP as the measurement marker for this study since it's one of the most used markers in synthetic biology and, as a result, most laboratories are equipped to measure this protein.

More

Calibration

OD600 Reference point

Measure the Abs600 of both the LUDOX CL-X (45% colloidal silica suspension) and water to obtain the correction factor.

Particle Standard Curve

Measure the Abs600 of a series of dilution monodisperse silica microspheres to draw the Particle Standard Curve.

Fluorescence standard curve

Measure the fluorescence of a series of diluted fluorescein to draw the fluorescein standard curve.

Cell measurement

We collaborate with the team SIAT-SCIE, because thire Distribution Kit was not delivered on time and we were during our final exam.
So we provide our kit and get the streaks of the transformed devices from them.

Histogram of Different Cultures’ Fluorescence at Each Time Point

Colony Forming Units

colonies: 1012

colonies: 133

colonies: 17

Summary

This year, according to the requirements of Measurement Committee, we measured the fluorescence data of E. coli strain DH5-alpha and obtained some relatively precise data. To be brief, we succeeded in reducing lab-to-lab variability in fluorescence measurements by normalizing to absolute cell count or colony-forming units (CFUs).

Feedback

In the protocol: Colony Forming Units per 0.1 OD600 E.coli cultures——Step 1: Starting Sample Preparation——2. Dilute your overnight culture to OD600...——Do This in triplicate for each culture , I think that should be added one more friendly reminder. That is, all cultures should be freezed in the ice in case the E.coli grows up quickly and influences the results of Step 3: CFU/mL/OD Calculation Instructions, in which we should have obtained a good data such as 1250, 125, 12, but acutually we had got some bad data like 1150, 988, 455 at the first measurement.

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+	h1, h2 {
+			color: #469789;
+		}
+</style>
+	<body data-spy="scroll" data-target="#myScrollspy" data-offset="10">
+		<div class="container-full">
+			<div class="card">
+				<img class="card-img-top" src="https://static.igem.org/mediawiki/2018/6/67/T--SZU-China--interlab.jpg" />
+			</div>
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 								<h1 id="header" class="text-center">InterLab Study</h1>
-								<p class="text-center text-success">"Measurement is fundamentally an act of communication." - Jacob Beal</p>
+								<p class="text-center" style="color:#469789 ;">"Measurement is fundamentally an act of communication." - Jacob Beal</p>
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 							</p>
 							<center>
-								<a href="https://2018.igem.org/Measurement/InterLab">More</a>
+								<a href="https://2018.igem.org/Measurement/InterLab" style="color:#469789 ;">More</a>
 							</center>
 						</div>
 					</div>
-					<div class="page-header">
+					<div class="indent">
 						<h2 id="Calibration">Calibration</h2>
-						<h4>OD600 Reference point</h4>
+						<h3>OD600 Reference point</h3>
 						<p>Measure the Abs600 of both the LUDOX CL-X (45% colloidal silica suspension) and water to obtain the correction factor. </p>
 						<div class="offset-1">
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 					</div>
-					<hr>
-					<h4>Particle Standard Curve</h4>
+					<div class="indent">
+						<h3>Particle Standard Curve</h3>
 					<p>Measure the Abs600 of a series of dilution monodisperse silica microspheres to draw the Particle Standard Curve.</p>
@@ Line 45: / Line 56: @@
 							</div>
+							<!--
 							<div class="card border-success mb-3">
 								<img class="card-img-top" src="https://static.igem.org/mediawiki/2018/4/48/T--SZU-China--InterLab_FSC_log.png" alt="card-img-cap" />
@@ Line 50: / Line 62: @@
 							</div>
+							-->
 						</div>
 					</div>
-					<hr>
+					</div>
-					<h4>Fluorescence standard curve</h4>
+					<div class="indent">
+						<h3>Fluorescence standard curve</h3>
 					<p>Measure the fluorescence of a series of diluted fluorescein to draw the fluorescein standard curve.</p>
 					<div class="row justify-content-center">
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 							</div>
+							<!--
 							<div class="card border-success mb-3">
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+					</div>
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-					<hr>
-					<h2 class="">Cell measurement</h2>
+					<div class="indent">
+						<h2 class="">Cell measurement</h2>
 					<p>
 						We collaborate with the team SIAT-SCIE, because thire Distribution Kit was not delivered on time and we were during our final exam.<br /> So we provide our kit and get the streaks of the transformed devices from them.
@@ Line 80: / Line 98: @@
 					<div class="row justify-content-center">
 						<div class="col-8">
+							<!--
 							<div class="card border-success mb-3">
 								<img width="512px" src="https://static.igem.org/mediawiki/2018/6/68/T--SZU-China--InterLab_Abs.jpg" />
 							</div>
+							-->
 							<div class="card border-success mb-3">
-								<img width="512px" src="https://static.igem.org/mediawiki/2018/3/30/T--SZU-China--InterLab_Flu.jpg" />
+								<img class="card-img-top" src="https://static.igem.org/mediawiki/2018/3/30/T--SZU-China--InterLab_Flu.jpg" />
 							</div>
+							<p class="text-center">
+								Histogram of Different Cultures’ Fluorescence at Each Time Point
+							</p>
 						</div>
 					</div>
+					</div>
-					<hr>
-					<h2>Colony Forming Units</h2>
+					<div class="indent">
+						<h2>Colony Forming Units</h2>
 					<div class="card-group">
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 							<img class="card-img-top" src="https://static.igem.org/mediawiki/2018/1/17/T--SZU-China--InterLab_CFU_1.png" alt="Card image cap" />
 							<div class="card-body">
-								<div class="card-title">CFU:1012</div>
+								<div class="card-title">colonies: 1012</div>
 							</div>
 						</div>
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 							<img class="card-img-top" src="https://static.igem.org/mediawiki/2018/3/37/T--SZU-China--InterLab_CFU_2.png" alt="Card image cap" />
 							<div class="card-body">
-								<div class="card-title">CFU:133</div>
+								<div class="card-title">colonies: 133</div>
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 						</div>
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 							<img class="card-img-top" src="https://static.igem.org/mediawiki/2018/c/c0/T--SZU-China--InterLab_CFU_3.png" alt="Card image cap" />
 							<div class="card-body">
-								<div class="card-title">CFU:17</div>
+								<div class="card-title">colonies: 17</div>
 							</div>
 						</div>
+					</div>
+					</div>
+					<div class="indent">
+						<h2>Summary</h2>
+						<p>This year, according to the requirements of Measurement Committee, we measured the fluorescence data of <i>E. coli</i> strain DH5-alpha and obtained some relatively precise data. To be brief, we succeeded in reducing lab-to-lab variability in fluorescence measurements by normalizing to absolute cell count or colony-forming units (CFUs).</p>
+					</div>
+					<div class="indent">
+						<h2>Feedback</h2>
+						<p>
+							In the protocol: <b>
+								Colony Forming Units per 0.1 OD600 E.coli cultures——Step 1: Starting Sample Preparation——2. Dilute your overnight culture to OD600...——Do This in triplicate for each culture
+							</b>, I think that should be added one more friendly reminder. That is, all cultures should be freezed in the ice in case the <i>E.coli</i> grows up quickly and influences the results of
+							<b>Step 3: CFU/mL/OD Calculation Instructions</b>, in which we should have obtained a good data such as 1250, 125, 12, but acutually we had got some bad data like 1150, 988, 455 at the first measurement.
+						</p>
 					</div>
@@ Line 124: / Line 165: @@
 	</body>
 </html>

Difference between revisions of "Team:SZU-China/InterLab"