Tracks/Measurement

From 2014.igem.org

(Difference between revisions)
(added main explanatory text for track)
Line 77: Line 77:
<tbody>
<tbody>
<tr>
<tr>
-
<td style="vertical-align: top;">Sample-mass-spec.png<br>
+
<td style="vertical-align: top;">
-
</td>
+
<center><img src="https://static.igem.org/mediawiki/2014/a/a0/Sample-mass-spec.png" style="width: 60%"></center><br>
-
<td style="vertical-align: top;">Flow_cytometry_sample.png<br>
+
A mass spectrometer can measure the amount of particular chemicals
-
</td>
+
-
</tr>
+
-
<tr>
+
-
<td style="vertical-align: top;">Microplate_reader.jpg<br>
+
-
<br>
+
-
</td>
+
-
<td style="vertical-align: top;">Microscopy_sample.jpg<br>
+
-
</td>
+
-
</tr>
+
-
</tbody>
+
-
</table>
+
-
<p>A mass spectrometer can measure the amount of particular chemicals
+
in a sample, but any cell measured is destroyed, it is difficult to
in a sample, but any cell measured is destroyed, it is difficult to
obtain measurement from individual cells, and often difficult to
obtain measurement from individual cells, and often difficult to
interpret the massive pattern of data produced to quantify particular
interpret the massive pattern of data produced to quantify particular
chemicals of interest.&nbsp; <br>
chemicals of interest.&nbsp; <br>
 +
</td>
 +
<td style="vertical-align: top;">
 +
<center><img src="https://static.igem.org/mediawiki/2014/3/34/Flow_cytometry_sample.png" style="width: 60%"></center><br>
A flow cytometer can take vast numbers of individual cell
A flow cytometer can take vast numbers of individual cell
measuremements, but the measurements are of a proxy fluorescent protein
measuremements, but the measurements are of a proxy fluorescent protein
Line 102: Line 93:
calibration controls are run with an experiment, the measurements are
calibration controls are run with an experiment, the measurements are
relative and non-reproducible.<br>
relative and non-reproducible.<br>
 +
</td>
 +
</tr>
 +
<tr>
 +
<td style="vertical-align: top;">
 +
<center><img src="https://static.igem.org/mediawiki/2014/6/67/Microplate_reader.jpg" style="width: 60%"></center><br>
A fluorimeter is less invasive than a flow cytometer and can measure
A fluorimeter is less invasive than a flow cytometer and can measure
changing fluorescence over time with little impact on the cells, but
changing fluorescence over time with little impact on the cells, but
Line 107: Line 103:
rather than individual cells, and also relative to the number of cells
rather than individual cells, and also relative to the number of cells
in the sample.<br>
in the sample.<br>
 +
</td>
 +
<td style="vertical-align: top;">
 +
<center><img src="https://static.igem.org/mediawiki/2014/a/a6/Microscopy_sample.jpg" style="width: 60%"></center><br>
A microscope can track and quantify fluorescence from individual cells,
A microscope can track and quantify fluorescence from individual cells,
but not very many of them, and often needs human help on tracking.<br>
but not very many of them, and often needs human help on tracking.<br>
-
</p>
+
</td>
-
<center><img src="https://static.igem.org/mediawiki/2014/3/38/Unit_mismatch.png" style="width: 60%"></center>
+
</tr>
-
<blockquote>
+
</tbody>
-
<b>Figure 2</b> Models using different relative units cannot be
+
</table>
-
compared or connected.&nbsp; How many "Blue" in the output characterized for
+
<blockquote><b>Figure 1</b>No generally available instrument can measure chemical concentrations in large number of single cells over time.</blockquote>
-
Repressor #1 are equal to a "Red" in the input characterized for
+
 
-
Repressor #2?<br>
+
-
</blockquote>
+
<p>Relative measurements are a major problem, because they cannot be
<p>Relative measurements are a major problem, because they cannot be
compared.&nbsp; If you build models of biological devices using
compared.&nbsp; If you build models of biological devices using
Line 127: Line 124:
been uniformly shifted (which might be very important!).<br>
been uniformly shifted (which might be very important!).<br>
</p>
</p>
 +
</p>
 +
<center><img src="https://static.igem.org/mediawiki/2014/3/38/Unit_mismatch.png" style="width: 60%"></center>
 +
<blockquote>
 +
<b>Figure 2</b> Models using different relative units cannot be
 +
compared or connected.&nbsp; How many "Blue" in the output characterized for
 +
Repressor #1 are equal to a "Red" in the input characterized for
 +
Repressor #2?<br>
 +
</blockquote>
<p>Beyond these core scientific concerns, there are pragmatic problems
<p>Beyond these core scientific concerns, there are pragmatic problems
as well. Instruments are also often very expensive to buy and to
as well. Instruments are also often very expensive to buy and to

Revision as of 22:37, 29 December 2013


iGEM 2014 Measurement New Track

Introduction

Precise measurements lie at the foundation of every scientific discipline, including synthetic biology. The limits of our knowledge are set by how well we can connect observations to reproducible quantities that give insight. Measurement is also an act of communication, allowing researchers to make meaningful comparisons between their observations. The science and technology of measurement are easily overlooked, because measuring devices are so familiar to us, but behind even the simplest devices lies an elaborate infrastructure. Consider a laboratory pipette. How accurate are the volumes it dispenses? How similar is it to other pipettes? How do you know? The answers to these questions are a complex story involving everything from the speed to light in vacuum to the atomic properties of cesium.

In synthetic biology, measurement is a critical challenge that is receiving and increasing amount of attention each year. For example, one of the long-standing goals of both iGEM and synthetic biology at large, is to characterize biological parts, so that they can be more easily used for designing new systems. The aim of the iGEM Measurement Track is to get students informed and excited about these problems, and to highlight the successes that teams are able to achieve in the area of measurement. The Measurement Track also aims to find out what measurement assays teams have available and to lay groundwork for future more complex measurement activities in iGEM.

Measurement Challenges in Synthetic Biology

With all the instruments in our laboratories, why isn't measurement a solved problem in synthetic biology?  Part of the problem is knowing what to measure and in what context.  One way to think about the impact of measurements is in terms of four levels, each building upon the last:

  1. Measurement quantifies a phenomenon that has been experimentally observed.
  2. Quantitative measurements are used to create a model of how the phenomenon was produced.
  3. Models are applied to predict what quantitative phenomena will be observed in a new context.
  4. Predictions are used to inform choices about how to engineer towards desired phenomena.
Instruments, by themselves, only address the first level.  In synthetic biology, many models are constructed, often post-facto. Quantitative predictions, however, are still extremely difficult: an important part of the problem is determining how measurement relates to context, so that we can understand what sorts of things a model can be reasonably expected to predict.

Even when we know what we wish to quantify, it may be impractical to obtain with our current instruments.  For example, many quantitative models are about how the concentration of chemicals in a single cell changes over time.  Behaviors often vary greatly from cell to cells, so it is often desirable to collect data from a large number of individual cells.  Most current instruments, however, cannot readily measure this.  Instead we end up having to make tradeoffs like these:


A mass spectrometer can measure the amount of particular chemicals in a sample, but any cell measured is destroyed, it is difficult to obtain measurement from individual cells, and often difficult to interpret the massive pattern of data produced to quantify particular chemicals of interest. 

A flow cytometer can take vast numbers of individual cell measuremements, but the measurements are of a proxy fluorescent protein rather than the actual chemical of interest and the cells may still be disrupted by running them through the instrument.  Unless calibration controls are run with an experiment, the measurements are relative and non-reproducible.

A fluorimeter is less invasive than a flow cytometer and can measure changing fluorescence over time with little impact on the cells, but still uses a proxy.  Its measurements are also of the whole sample rather than individual cells, and also relative to the number of cells in the sample.

A microscope can track and quantify fluorescence from individual cells, but not very many of them, and often needs human help on tracking.
Figure 1No generally available instrument can measure chemical concentrations in large number of single cells over time.

Relative measurements are a major problem, because they cannot be compared.  If you build models of biological devices using different relative measurements, then you cannot combine the models to predict what will happen when you combine the devices.  If units are relative to a batch of samples or to a laboratory, then you cannot reproduce experimental results: even if two experiments produce the same numbers in a new experiment, if the units are relative you cannot tell whether the results are actually the same or whether they have been uniformly shifted (which might be very important!).

Figure 2 Models using different relative units cannot be compared or connected.  How many "Blue" in the output characterized for Repressor #1 are equal to a "Red" in the input characterized for Repressor #2?

Beyond these core scientific concerns, there are pragmatic problems as well. Instruments are also often very expensive to buy and to operate.  This is an especially big problem for DIY groups and researchers in smaller institutions or developing nations.  Cheaper instruments are sometimes available, but usually produce much less accurate or precise data.  Once you've got the data, you also need to be able to share it effectively, so that everybody can benefit from the information that is being learned.  The community will thus likely also need new tools and data exchange standards to allow for simpler and more effective sharing of measurements and models.

The challenges of measurement in synthetic biology are large and broad.  They cover everything from fundamental biological questions to the need for better cheaper instruments and community data sharing.  But because measurement affects to many things, improvements in any of these areas are likely to have a big impact.

Additional Reading on Measurement and Synthetic Biology

Here are some additional resources that may be interesting and can help you learn more about the lay of the land for measurement in synthetic biology:

Readings on Instruments and Metrology
Readings on Device Characterization
Agilent Measurement 101
Relative Promoter Units
NIST cross-lab
TASBE protocols for flow cytometry calibration and part characterization
NIST study on flow cytometer calibration beads
Proposed "datasheet" for BBxxxx
SpheroTech Beads


Plans for the Measurement Track in 2014

The 2014 event expands on iGEM's long-running inclusion of measurement as a focus area (a measurement award has been given since 2006).  This year we are introducing a medal for measurement, and splitting the single prior award into two awards.

Teams participating in the Measurement Track in 2014 can earn a medal by taking part in a group measurement project, in which each team measures the same properties of several known samples.  We will provide some recommendations for experimental and measurement protocols, but teams are encouraged to use whatever approach will provide the most reliable and accurate measurements with the resources available to them.  All of the results will be collected together by iGEM HQ and later shared, which will allow people to see the tradeoffs between different approaches.

Teams will also be able to compete for two awards:

  • Best Characterization Project focuses on performing measurement.  It will be awarded to the team that best gathers of high-quality data about the behavior of biological devices that can aid future engineering projects.
  • Best Innovation in Measurement focuses on improving measurement.  It will be awarded to the team that provides the best improvement to quality and/or accessibility of measurement techniques.

Measurement Track Committee

We have a great committee to help coordinate the Measurement track in 2014.

  1. Chair: Jacob Beal, Raytheon BBN Technologies
  2. Traci Haddock, Boston University
  3. Jim Hollenhorst, Agilent Technologies