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Difference between revisions of "Talk:O2k-Fluo LED2-Module"

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Previous Product ID 34000-01
== Measuring hydrogen peroxide ==
* [[Measuring hydrogen peroxide]]


== Simultaneous measurement of TPP and fluorescence ==


'''Question:''' Will it be possible to measure JO2, fluorescence AND TPP simultaneously, or just JO2/fluorescence vs JO2/TPP?
== Older series ==


=== O2k Series A to C ===


'''Answer:''' Background
* The Oxygraph-2k [[O2k-Main Unit#O2k-Series|Series]] A to C do not support the O2k-Fluo LED2-Module. We thank you for your understanding.
The main unknown is the chemical compatibility of the methods. We still have to find out whats the effect of Amplex red and its reaction product on the TPP signal.
If this is not a big problem there are technical issues: a black TPP stopper will be required and then still light entering the chamber through the TPP electrode might be a problem. Producing the TPP electrodes in black is presumable not a very good idea because then it will no longer be possible to "see" the position of the membrane. I think the technical problems are solvable but first we have to check for chemical compatibility.


'''Update:'''
First exploratory experiment:


A chamber was equipped with TPP electrodes (black stoppers) and a fluorescence module for measuring H2O2 via the Amplex Red method. A standard TPP calibration was carried out.
=== O2k-Fluo LED2-Module, Series A ===
Amplex red / HRP addition resulted only in a minor signal in the TPP channel, a further TPP calibration showed no obvious large negative effects on the performance of the TPP electrode. An H2O2 calibration of the fluorescence signal was carried out: The '''sensitivity''' for H2O2 was reducedย  by a '''factor of 3 to 4''' as compared toย  measurements without TPP electrodes. At the same time the noiseย  was drastically increased. In the comparative experiment (without TPP electrodes) no random noise was seen - digital resolution was the limiting factor. Based on this comparison, '''noise''' increased in the experiment with TPP electrodes at least by a '''factor of 20''', probable more.
It will be possible to estimate this factor with a higher precision after running an experiment without TPP electrodes at a higher gain (higher digital resolution).


It was further tested whether the presence of TPP+ alone (without electrodes) could explain this behavior but, if there were any effects at all, they were quite small.
''' Setting the LED intensity directly at the Fluorescence-Control Unit'''
Useย  the small supplied screwdriver to change the position of the switch on the front panel of the O2k-Fluo Control Unit, using the table below:


Peroxide additions corresponding to a concentration change of 110 nM (110 pmol/ml) were still well visible but not additions corresponding to a 22 nM (22 pmol/ml) concentration change.
{| class="wikitable" style="text-align: center;"
|-
! Position
! scope="col" width="20" |0
! 1
! scope="col" width="20" |2
! scope="col" width="20" |3
! scope="col" width="20" |4
! scope="col" width="20" |5
! scope="col" width="20" |6
! scope="col" width="20" |7
! scope="col" width="20" |8
! 9
|-
! scope="row"| LED current [mA]
|| off || 0.02 || 0.5 || 1|| 2|| 5|| 10|| 20|| 30|| set by DatLab
|}


This was only one exploratory experiment (2 chambers)!


Based on this preliminary data:
[[Image:BB-Bioblast.jpg|left|40px|link=http://www.bioblast.at/index.php/Bioblast:About |Bioblast wiki]]
An important point is why one would want to measure TPP and H2O2 simultaneously in the same chamber: If this is "only" for time / sample economy the results above strongly discourage this idea. Parallel measurement e.g one chamber TPP / one chamber H2O2 are preferable. ย 
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If there is a very strong need to measure both parameters on the same sample (e.g. if strong in-homogeneity among samples in this respect is suspected) and a comparable high H2O2 flux is expected the simultaneous measurement might be principally doable, especially if further optimizations are possible. E.g.: Maybe with the TPP electrode in the chamber black stirrers become important again? However, this certainly would involve some methodological work and the results would be second class at the best.
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== Coupling the O2k to optical instruments: Geometry ==
ย 
For various analytical techniques it is desired to couple optical sensors and light sources to the O2k chamber. The initial approach to do so was to insert the optical probe via a custom designed black stopper from above directly into the chamber, see โ€ฆ This approach (light and detection from above) requires also the use of black stirrer
However, in Tony Hickey's ([[Hickey 2012 J Comp Physiol B]]) and in our own development of the fluorescence module ([[Fasching 2011 Abstract Berlin]]ย  it became clear that for most applications in the visible range it is a better and easier strategy to introduce the light via the front window and detect the light via the same way. The Duran glass of the O2k chamber has very high transmission down to at least 350 nm and is probable usable even further down, see [http://www.duran-group.com/en/about-duran/duran-properties/optical-properties-of-duran.html Duran optical properties ]
The โ€œvia the windowโ€ approach has several important benefits:
# the optical sensor does not โ€œseeโ€ the stirrers. Therefore, for comparable small optical sensor diameters there was no need to use black stirrers. In fact using white stirrers increased overall sensitivity without introducing any disturbances.
# no physical contact of the sample with the optical sensor necessary
# the space on top of the stopper is not taken up by the optical sensor, allowing for easier titrations and at least potentially for simultaneous use of additional electrodes introduced via the stopper
The black but otherwise regular stopper is required to shield the chamber from outside light.
Development with this approach was facilitated by the (rather lucky) fact that the diameter of the O2k chamber window is identical to the chamber diameter, therefore a stopper with o-ring designed to be introduced into the chamber from above, can also be placed in the chamber window for initial experiments. As a permanent, final sensor a more stable solution should be used however.
We used this configuration not only with our LED based fluorescence module but also to couple a full spectrofluorometer to the O2k chamber.
We think this might be worth to try also for these groups that need a full spectrofluorometer or other light guide based detectors / sourcesย  attached to the oxygraph.
--[[User:Fasching Mario|Fasching Mario]] 09:26, 17 February 2012 (CET)
ย 
== Oxygraph Series A to C ==
ย 
*The Oxygraph-2k, [[O2k-Main Unit#O2k-Series|Series]] A to C, can currently not be equipped with an O2k-Fluorescence LED2-Module. We thank you for your understanding.
ย 
ย 
[[User:Fasching Mario|Fasching Mario]] 11:55, 25 January 2012 (CET)

Latest revision as of 16:11, 11 December 2019

Previous Product ID 34000-01


Older series

O2k Series A to C

  • The Oxygraph-2k Series A to C do not support the O2k-Fluo LED2-Module. We thank you for your understanding.


O2k-Fluo LED2-Module, Series A

Setting the LED intensity directly at the Fluorescence-Control Unit Use the small supplied screwdriver to change the position of the switch on the front panel of the O2k-Fluo Control Unit, using the table below:

Position 0 1 2 3 4 5 6 7 8 9
LED current [mA] off 0.02 0.5 1 2 5 10 20 30 set by DatLab


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