Deconvolving Spinning Disk Images

> Commercial Response from Media Cybernetics:
>
> I'm a software developer on the Autoquant product.
>
> 2.  The issue is not strictly theoretical vs. calculated but more of a question of how well you can measure or calculate the PSF.  For measured the issue is getting a picture of a bead under the same conditions (depth and RI) as the sample.  For theoretical it is knowing the values of the depth and sample RI.  Can you get a picture of a bead under conditions similar to the real experiment?? Or alternatively do you know a good estimate of depth and sample RI?? Both can be tricky.
>
> And actually MLE can be used with theoretical PSFs.  You may be thinking of the adaptive PSF MLE in Autoquant.  It's a version of MLE in which the PSF is allowed to change (subject to constraints).  Adaptive MLE uses a theoretical or measured PSF as a starting point.  Autoquant also has routines to detect spherical aberration (which can be problematic with thick samples).
>
> Please feel free to contact us off list if you have any further questions.
>
>
>
> -----Original Message-----
> From: Confocal Microscopy List [mailto:[hidden email]] On Behalf Of Dani
> Sent: Thursday, June 23, 2011 10:22 AM
> To: [hidden email]
> Subject: Deconvolving Spinning Disk Images
>
> *****
> To join, leave or search the confocal microscopy listserv, go to:
> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> *****
>
> Hi there,
>
> I would like to deconvolve my spinning disk images for quantification
> purposes. Regarding this, I have a few issues/questions.
>
> 1. I have been trying to image fluorescent beads, in order to obtain PSF
> measurements for my microscope (conditions). However, whenever I do this, I
> always “see the grid” of the spinning disk unit, meaning that there are
> multiple points visible at the same time, even when a single bead is imaged.
> This only becomes obvious after severe rescaling and the other grid dots
> have a very weak intensity compared to the main dot (at least 2 orders of
> magnitude). I have tried synchronizing imaging time with spinning disk
> speed, long/short exposures, high/low laser intensities, with/without EM
> gain, etc. I always see the same thing.
> The questions are: Will this affect the deconvolution efficiency/accuracy?
> Does anyone have any solution for this problem?
>
>
>
> 2. I have read conflicting opinions on performing deconvolution using
> experimental vs. theoretical PSFs vs maximum likelihood estimations (MLE).
> Some say that when imaging thick samples (in my case ~30um) it is better to
> do MLEs, because the PSF changes depending on the depth that you image, and
> measured PSFs are always on the surface of the slide. Others say that
> measured PSFs will always (usually) be better as they don’t assume anything
> but actually measure what is going on. Then again, I have been considering
> doing theoretical PSFs, as I have been having a lot of trouble actually
> measuring a proper PSF in my microscope (see point 1).
> Does anyone have any experience with this or can advise me on these issues.
> Which programs/algorithms/plugins could I best use for this?
>
>
> --
> View this message in context: http://confocal-microscopy-list.588098.n2.nabble.com/Deconvolving-Spinning-Disk-Images-tp6508446p6508446.html
> Sent from the Confocal Microscopy List mailing list archive at Nabble.com.
>
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> *****
> To join, leave or search the confocal microscopy listserv, go to:
> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> *****
>
> Hi there,
>
> I would like to deconvolve my spinning disk images for quantification
> purposes. Regarding this, I have a few issues/questions.
>
> 1. I have been trying to image fluorescent beads, in order to obtain PSF
> measurements for my microscope (conditions). However, whenever I do this,
> I
> always “see the grid” of the spinning disk unit, meaning that there are
> multiple points visible at the same time, even when a single bead is
> imaged.
> This only becomes obvious after severe rescaling and the other grid dots
> have a very weak intensity compared to the main dot (at least 2 orders of
> magnitude). I have tried synchronizing imaging time with spinning disk
> speed, long/short exposures, high/low laser intensities, with/without EM
> gain, etc. I always see the same thing.
> The questions are: Will this affect the deconvolution efficiency/accuracy?
> Does anyone have any solution for this problem?
>
>
>
> 2. I have read conflicting opinions on performing deconvolution using
> experimental vs. theoretical PSFs vs maximum likelihood estimations (MLE).
> Some say that when imaging thick samples (in my case ~30um) it is better
> to
> do MLEs, because the PSF changes depending on the depth that you image,
> and
> measured PSFs are always on the surface of the slide. Others say that
> measured PSFs will always (usually) be better as they don’t assume
> anything
> but actually measure what is going on. Then again, I have been considering
> doing theoretical PSFs, as I have been having a lot of trouble actually
> measuring a proper PSF in my microscope (see point 1).
> Does anyone have any experience with this or can advise me on these
> issues.
> Which programs/algorithms/plugins could I best use for this?
>
>
> --
> View this message in context:
> http://confocal-microscopy-list.588098.n2.nabble.com/Deconvolving-Spinning-Disk-Images-tp6508446p6508446.html
> Sent from the Confocal Microscopy List mailing list archive at Nabble.com.

>*****
>To join, leave or search the confocal microscopy listserv, go to:
>http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
>*****
>
>Hello,
>
>it seems to me that you are dealing with the
>common problem of pinhole cross talk, in which
>the neighboring pinholes contribute in such way
>that your PSF will contain next to the main peak
>about six more of lesser intensity around it. To
>deconvolve such image, you need this patterned
>PSF! If you want to use a theoretical PSF you
>need to work out the exact forward problem and
>then generate a PSF that matches your instrument
>in all parameters especially the geometry of the
>cross-talking pinholes. Working with blind
>deconvolution might be tricky, as there are
>often heavy constraints on the PSF to introduce
>additional knowledge. Unless your blind
>deconvolution system supports such crosstalk
>PSF's, I would not resort to this option.
>Finally you can try to acquire an empirical PSF
>using a small bead. The caveat is, that you can
>only use a bead that is far enough away from
>others so that it does not interfere with the
>crosstalk pattern of other beads. Then, you just
>cut out and center this single bead stack and
>use it for deconvolution.
>
>hope it helped
>regards
>Lutz
>
>__________________________________
>L u t z   S c h a e f e r
>Sen. Scientist
>Mathematical modeling / Image processing
>Advanced Imaging Methodology Consultation
>16-715 Doon Village Rd.
>Kitchener, ON, N2P 2A2, Canada
>Phone/Fax: +1 519 894 8870
>Email:     [hidden email]
>___________________________________
>
>--------------------------------------------------
>From: "Dani" <[hidden email]>
>Sent: Thursday, June 23, 2011 10:22
>To: <[hidden email]>
>Subject: Deconvolving Spinning Disk Images
>
>>*****
>>To join, leave or search the confocal microscopy listserv, go to:
>>http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
>>*****
>>
>>Hi there,
>>
>>I would like to deconvolve my spinning disk images for quantification
>>purposes. Regarding this, I have a few issues/questions.
>>
>>1. I have been trying to image fluorescent beads, in order to obtain PSF
>>measurements for my microscope (conditions). However, whenever I do this, I
>>always "see the grid" of the spinning disk unit, meaning that there are
>>multiple points visible at the same time, even when a single bead is imaged.
>>This only becomes obvious after severe rescaling and the other grid dots
>>have a very weak intensity compared to the main dot (at least 2 orders of
>>magnitude). I have tried synchronizing imaging time with spinning disk
>>speed, long/short exposures, high/low laser intensities, with/without EM
>>gain, etc. I always see the same thing.
>>The questions are: Will this affect the deconvolution efficiency/accuracy?
>>Does anyone have any solution for this problem?
>>
>>
>>
>>2. I have read conflicting opinions on performing deconvolution using
>>experimental vs. theoretical PSFs vs maximum likelihood estimations (MLE).
>>Some say that when imaging thick samples (in my case ~30um) it is better to
>>do MLEs, because the PSF changes depending on the depth that you image, and
>>measured PSFs are always on the surface of the slide. Others say that
>>measured PSFs will always (usually) be better as they don't assume anything
>>but actually measure what is going on. Then again, I have been considering
>>doing theoretical PSFs, as I have been having a lot of trouble actually
>>measuring a proper PSF in my microscope (see point 1).
>>Does anyone have any experience with this or can advise me on these issues.
>>Which programs/algorithms/plugins could I best use for this?
>>
>>
>>--
>>View this message in context:
>>http://confocal-microscopy-list.588098.n2.nabble.com/Deconvolving-Spinning-Disk-Images-tp6508446p6508446.html
>>Sent from the Confocal Microscopy List mailing list archive at Nabble.com.

> *****
> To join, leave or search the confocal microscopy listserv, go to:
> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> *****
>
> Well, what Lutz says is precisely true, but on
> the other hand, unless the stained part of the
> specimen is quite thick, it may not be very
> important.
>
> Yes, light that originates far from the focus
> plane may come through the wrong pinhole. As the
> pinhole in an image plane it will actually arrive
> at the CCD in the wrong location. But on the
> other hand, it isn't very much light. In the
> Yoko, where the pinholes are 50µm and 250µm
> apart, the circle of transmission where the first
> light would come through has a circumference
> about 1570 µm (of which at most 6x50 or 300 µmm
> is open, more likely about 200 µm),  a diameter
> of 500 µm and an area of about 200k square
> microns. Of this, about 8000 square microns is
> "hole", about 4%. Apart from the geometry, the
> light focused back from the "spot" in the
> specimen tends to cluster near the pinhole, so
> the fraction of this out-of-focus light
> prohibited from reaching the detector is probably
> more than 96 parts out of 100.
>
> It is then important to remember that this is a
> confocal microscope, and we often only get very
> few photons through the pinhole in any case
> (maybe tens-hundreds  in a 1 sec exposure) and "a
> lot less that very few is close to zero" if you
> will permit the imprecision.
>
> The z-resolution of disc scanners was much
> studied when they first came out and the Z-image
> of a plane of fluorophor is almost the same as a
> single point scanner(with the same pinhole size)
> with the exception that when the focus plane
> moves far from focus, the signal level does not
> asymptote to zero, but to the amount of light
> that would pass an ND filter with the same
> average transmission as the disk. Other stain
> distributions may be produce other results (a
> periodic structure that appeared in the plane of
> the disk with a period that matched that of the
> hole pattern for instance) but it is not beyond
> the wit of man to obtain and use a measured 3D
> PSF to deconvolve confocal data of any type,
> including disc scanners.
>
> I recommend it.
>
> JP
>
>
>> *****
>> To join, leave or search the confocal microscopy listserv, go to:
>> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
>> *****
>>
>> Hello,
>>
>> it seems to me that you are dealing with the
>> common problem of pinhole cross talk, in which
>> the neighboring pinholes contribute in such way
>> that your PSF will contain next to the main peak
>> about six more of lesser intensity around it. To
>> deconvolve such image, you need this patterned
>> PSF! If you want to use a theoretical PSF you
>> need to work out the exact forward problem and
>> then generate a PSF that matches your instrument
>> in all parameters especially the geometry of the
>> cross-talking pinholes. Working with blind
>> deconvolution might be tricky, as there are
>> often heavy constraints on the PSF to introduce
>> additional knowledge. Unless your blind
>> deconvolution system supports such crosstalk
>> PSF's, I would not resort to this option.
>> Finally you can try to acquire an empirical PSF
>> using a small bead. The caveat is, that you can
>> only use a bead that is far enough away from
>> others so that it does not interfere with the
>> crosstalk pattern of other beads. Then, you just
>> cut out and center this single bead stack and
>> use it for deconvolution.
>>
>> hope it helped
>> regards
>> Lutz
>>
>> __________________________________
>> L u t z   S c h a e f e r
>> Sen. Scientist
>> Mathematical modeling / Image processing
>> Advanced Imaging Methodology Consultation
>> 16-715 Doon Village Rd.
>> Kitchener, ON, N2P 2A2, Canada
>> Phone/Fax: +1 519 894 8870
>> Email:     [hidden email]
>> ___________________________________
>>
>> --------------------------------------------------
>> From: "Dani" <[hidden email]>
>> Sent: Thursday, June 23, 2011 10:22
>> To: <[hidden email]>
>> Subject: Deconvolving Spinning Disk Images
>>
>>> *****
>>> To join, leave or search the confocal microscopy listserv, go to:
>>> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
>>> *****
>>>
>>> Hi there,
>>>
>>> I would like to deconvolve my spinning disk images for quantification
>>> purposes. Regarding this, I have a few issues/questions.
>>>
>>> 1. I have been trying to image fluorescent beads, in order to obtain PSF
>>> measurements for my microscope (conditions). However, whenever I do this, I
>>> always "see the grid" of the spinning disk unit, meaning that there are
>>> multiple points visible at the same time, even when a single bead is imaged.
>>> This only becomes obvious after severe rescaling and the other grid dots
>>> have a very weak intensity compared to the main dot (at least 2 orders of
>>> magnitude). I have tried synchronizing imaging time with spinning disk
>>> speed, long/short exposures, high/low laser intensities, with/without EM
>>> gain, etc. I always see the same thing.
>>> The questions are: Will this affect the deconvolution efficiency/accuracy?
>>> Does anyone have any solution for this problem?
>>>
>>>
>>>
>>> 2. I have read conflicting opinions on performing deconvolution using
>>> experimental vs. theoretical PSFs vs maximum likelihood estimations (MLE).
>>> Some say that when imaging thick samples (in my case ~30um) it is better to
>>> do MLEs, because the PSF changes depending on the depth that you image, and
>>> measured PSFs are always on the surface of the slide. Others say that
>>> measured PSFs will always (usually) be better as they don't assume anything
>>> but actually measure what is going on. Then again, I have been considering
>>> doing theoretical PSFs, as I have been having a lot of trouble actually
>>> measuring a proper PSF in my microscope (see point 1).
>>> Does anyone have any experience with this or can advise me on these issues.
>>> Which programs/algorithms/plugins could I best use for this?
>>>
>>>
>>> --
>>> View this message in context:
>>> http://confocal-microscopy-list.588098.n2.nabble.com/Deconvolving-Spinning-D
>>> isk-Images-tp6508446p6508446.html
>>> Sent from the Confocal Microscopy List mailing list archive at Nabble.com.
>
>
> --
>                     ****************************************
> Prof. James B. Pawley,                                     Phone: 604-822-7801
> 3D Microscopy of Living Cells: Summer Course   CELL: 778-919-3176
> Info at: http://www.3dcourse.ubc.ca
> "If it isn't diffraction, it is statistics":Microscopist's complaint, Anon.

> *****
> To join, leave or search the confocal microscopy listserv, go to:
> http://lists.umn.edu/cgi-bin/**wa?A0=confocalmicroscopy<http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy>
> *****
>
> Hello Dear Listers,
>
> We have run into a conundrum regarding live, semi-long term and fixable
> labelling of two population of mouse ES cells for aggregation/sorting out
> studies.
> We would like to fix label cells (two cell strains), let them aggregate,
> fix the aggregates after 3-4 days and be able to make them out with either
> am ancient Bio-Rad MRC 600 Krypton/Argon (488, 568 and 647 nm) or
> a prehistorical Zeiss Photomicroscope (DAPI/Hoechst @ ~350 nm, FITC @ ~390
> nm and TRITC (~440 nm) ot Texas Red (~620 nm).
>
> Invitrogen/Molecular Probes (http://www.invitrogen.com/**
> site/us/en/home/References/**Molecular-Probes-The-Handbook/**
> Fluorescent-Tracers-of-Cell-**Morphology-and-Fluid-Flow/**
> Membrane-Permeant-Reactive-**Tracers.html#head2<http://www.invitrogen.com/site/us/en/home/References/Molecular-Probes-The-Handbook/Fluorescent-Tracers-of-Cell-Morphology-and-Fluid-Flow/Membrane-Permeant-Reactive-Tracers.html#head2>)
> offer quite few cell tracking probes but figuring out what does what is
> difficult (for me, at least).
> They say that CellTracker Green CMFDA (5-chloromethylfluorescein diacetate)
> labels cells that are both fluorescent and viable for at least 24 hours
> after loading.
> We need three-four days, though.
> Orange-fluorescent CellTracker Orange CMRA  - ditto.
>
> CellTrace Oregon Green 488 Carboxylic Acid Diacetate Succinimidyl Ester is
> highly recommended but nothing is said of its fixability.
> It is said that CellTrace Far Red DDAO-SE is a fixable, far-red–fluorescent
> tracer for long-term cell labelling but from the literature given I am not
> sure of its longevity.
>
> Sigma (http://www.sigmaaldrich.com/**img/assets/8200/PKH_LinkerKit_**
> web_version.pdf<http://www.sigmaaldrich.com/img/assets/8200/PKH_LinkerKit_web_version.pdf>)
> sells PKH26 and PKH67 that (Sigma says) are stable for up to 100 days in
> vivo (PKH26), but I do not see them heavily used in cell tracking other than
> FACS.
>
> /Ergo/,
> Any practical suggestion shall be greatly appreciated!
>
> Greetings,
>
> Michal
>
> PS
> Obviously (and to my chagrin) I have no financial association with neither
> company.
> M.O.
>

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> *****
>
> Right!
> Thanks Joel,
>
> Michal
>

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> *****
>
> Right!
> Thanks Joel,
>
> Michal
>