averaging vs. accumulation for noise reduction - is there a difference?

> *****
> To join, leave or search the confocal microscopy listserv, go to:
> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> *****
>
> Hallo,
> this is a very basic question, but I cannot figure this out from what I have
> been reading, so a simple explanation for a non-physicist would be much
> appreciated:
>
> Is there a real difference in the improvement of the signal to noise ratio
> between frame averaging (or accumulation) and longer dwell times (slower
> scan) for a point-scanning confocal witrh a PMT detector?
>
> For instance, using single point scanning confocal, 12-bit acquisition.
>
> a) averaging (or accumulating) 5 frames, 4 microseconds per pixel
> b) acquiring a single frame, 20 microseconds per pixel
>
> Assumptions:
> no saturation of the detector;
> stable environmental conditions, no focus drift, etc
>
> Would it matter (for the dfference between the two scenarios) if it was analog
> detection or photon counting detection?
>
> I will run this little test later, but I am curious what you think.
>
> I thought that at least for the photon counting mode, the two important
> factors would be the dark counts and the total number of counts detected, so
> whether it is acquired in one scan or in 5 scans, it should be the same. My
> camera expert here insists that the averaging scheme will give better noise
> suppression.
>
> Thanks!
>
>
> Stan Vitha  
>
> Microscopy and Imaging Center
> Texas A&M University

>
>
>
> Brian Armstrong PhD
> Light Microscopy Core
> Beckman Research Institute
> 1450 East Duarte Rd
> Duarte, CA 91010
> 626-256-4673 x62872
>

> --
> Julio Vazquez
> Fred Hutchinson Cancer Research Center
> Seattle, WA
>
> http://www.fhcrc.org/
>
>
> On Jun 16, 2011, at 2:08 PM, Moninger, Thomas wrote:
>
>> Stan,
>>
>> I've been told by Carl Z. engineers that in general averaging (I usually

>
>
>
> Brian Armstrong PhD
> Light Microscopy Core
> Beckman Research Institute
> 1450 East Duarte Rd
> Duarte, CA 91010
> 626-256-4673 x62872
>

> --
> Julio Vazquez
> Fred Hutchinson Cancer Research Center
> Seattle, WA
>
> http://www.fhcrc.org/
>
>
> On Jun 16, 2011, at 2:08 PM, Moninger, Thomas wrote:
>
>> Stan,
>>
>> I've been told by Carl Z. engineers that in general averaging (I

> *****
> To join, leave or search the confocal microscopy listserv, go to:
> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> *****
>
> Hallo,
> this is a very basic question, but I cannot figure this out from what I have
> been reading, so a simple explanation for a non-physicist would be much
> appreciated:
>
> Is there a real difference in the improvement of the signal to noise ratio
> between frame averaging (or accumulation) and longer dwell times (slower
> scan) for a point-scanning confocal witrh a PMT detector?
>
> For instance, using single point scanning confocal, 12-bit acquisition.
>
> a) averaging (or accumulating) 5 frames, 4 microseconds per pixel
> b) acquiring a single frame, 20 microseconds per pixel
>
> Assumptions:
> no saturation of the detector;
> stable environmental conditions, no focus drift, etc
>
> Would it matter (for the dfference between the two scenarios) if it was analog
> detection or photon counting detection?
>
> I will run this little test later, but I am curious what you think.
>
> I thought that at least for the photon counting mode, the two important
> factors would be the dark counts and the total number of counts detected, so
> whether it is acquired in one scan or in 5 scans, it should be the same. My
> camera expert here insists that the averaging scheme will give better noise
> suppression.
>
> Thanks!
>
>
> Stan Vitha
>
> Microscopy and Imaging Center
> Texas A&M University
>
>    

>To join, leave or search the confocal microscopy listserv, go to:
>http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
>*****
>
>I agree with Julio and Brian about the Zeiss 510 - averaged images were
>always less noisy than "dwelled" images.  I always taught that point in
>training sessions and showed side by side comparisons; newbies could clearly
>see the benefit of averaging over dwelling.  However this isn't the case on
>my 710 or 700, I see no difference (just by eye!) between averaging and
>dwelling (~800 volt gain comparing 4-8 averages to dwell times 4-8x slower
>than whatever max. is [1~3 us]).
>
>-Esteban
>
>
>On Thu, Jun 16, 2011 at 2:38 PM, Armstrong, Brian <[hidden email]>
>wrote:
>>  *****
>>  To join, leave or search the confocal microscopy listserv, go to:
>>  http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
>>  *****
>>
>>  I have not done a careful analysis of this either, and I am not quite sure
>how you would, however I share the viewpoint of Julio exactly, 1.6usec/pix
>and 2-4 ave.
>>
>>
>>
>>  Brian Armstrong PhD
>>  Light Microscopy Core
>>  Beckman Research Institute
>>  1450 East Duarte Rd
>>  Duarte, CA 91010
>>  626-256-4673 x62872
>>
>http://www.cityofhope.org/SharedResources/LightMicroscopy/LightMicroHome.htm
>>
>>
>>  -----Original Message-----
>>  From: Confocal Microscopy List [mailto:[hidden email]]
>On Behalf Of Julio Vazquez
>>  Sent: Thursday, June 16, 2011 2:21 PM
>>  To: [hidden email]
>>  Subject: Re: averaging vs. accumulation for noise reduction - is there a
>difference?
>>
>>  *****
>>  To join, leave or search the confocal microscopy listserv, go to:
>>  http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
>>  *****
>>
>>  This is what I noticed empirically on our Zeiss LSM 510, where averaging
>tends to give somewhat better noise reduction than increasing dwell time.
>Under "normal" imaging conditions, we typically use a dwell time of 1.6-3.2
>microseconds. Increasing the dwell time to greater than  3.2 microseconds
>tends to result in more bleaching and somewhat reduced signal. Typically, we
>use 1.6 microseconds dwell time, and 2-4 averages, depending on the sample.
>>  --
>>  Julio Vazquez
>>  Fred Hutchinson Cancer Research Center
>>  Seattle, WA
>>
>>  http://www.fhcrc.org/
>>
>>
>>  On Jun 16, 2011, at 2:08 PM, Moninger, Thomas wrote:
>>
>>>  Stan,
>>>
>>>  I've been told by Carl Z. engineers that in general averaging (I usually
>use line, not frame) tends to yield better S/N then does increasing dwell
>time. As Lloyd commented this may be model specific. I have not done any
>analysis to confirm this however....
>>>
>>>  Tom
>>
>>
>>  ---------------------------------------------------------------------
>>  SECURITY/CONFIDENTIALITY WARNING:
>>  This message and any attachments are intended solely for the individual or
>entity to which they are addressed. This communication may contain
>information that is privileged, confidential, or exempt from disclosure
>under applicable law (e.g., personal health information, research data,
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>view the information, forward it to others or tamper with the information
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>>

>than whatever max. is [1~3 us]).
>
>-Esteban
>
>
>On Thu, Jun 16, 2011 at 2:38 PM, Armstrong, Brian <[hidden email]>
>wrote:
>>  *****
>>  To join, leave or search the confocal microscopy listserv, go to:
>>  http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
>>  *****
>>
>>  I have not done a careful analysis of this either, and I am not

>and 2-4 ave.
>>
>>
>>
>>  Brian Armstrong PhD
>>  Light Microscopy Core
>>  Beckman Research Institute
>>  1450 East Duarte Rd
>>  Duarte, CA 91010
>>  626-256-4673 x62872
>>
>http://www.cityofhope.org/SharedResources/LightMicroscopy/LightMicroHom

>>  --
>>  Julio Vazquez
>>  Fred Hutchinson Cancer Research Center
>>  Seattle, WA
>>
>>  http://www.fhcrc.org/
>>
>>
>>  On Jun 16, 2011, at 2:08 PM, Moninger, Thomas wrote:
>>
>>>  Stan,
>>>
>>>  I've been told by Carl Z. engineers that in general averaging (I

> *****
> To join, leave or search the confocal microscopy listserv, go to:
> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> *****
>
> I was talking about sub-pixel scan inaccuracy, which would not be
> sufficient to cause visible blurring but could give some smoothing.
>
> Image 'brightness', mentioned by another contributor to this thread, is
> not a meaningful figure (particularly without any figures quoted).  For
> example, resonant scans might be digitized at 8-bit for the sake of
> speed, and non-resonant ones at 12 bit.  Brightness is then just a
> function of the display algorithm.
>
>                     Guy
>
>
> Optical Imaging Techniques in Cell Biology
> by Guy Cox    CRC Press / Taylor&  Francis
>       http://www.guycox.com/optical.htm
> ______________________________________________
> Associate Professor Guy Cox, MA, DPhil(Oxon)
> Australian Centre for Microscopy&  Microanalysis,
> Madsen Building F09, University of Sydney, NSW 2006
>
> Phone +61 2 9351 3176     Fax +61 2 9351 7682
>               Mobile 0413 281 861
> ______________________________________________
>        http://www.guycox.net
>
>
>
> -----Original Message-----
> From: Confocal Microscopy List [mailto:[hidden email]]
> On Behalf Of James Pawley
> Sent: Friday, 17 June 2011 3:36 PM
> To: [hidden email]
> Subject: Re: averaging vs. accumulation for noise reduction - is there a
> difference?
>
> *****
> To join, leave or search the confocal microscopy listserv, go to:
> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> *****
>
> Hi all,
>
> I haven't seen these images but the "dwell" image (slower scan?)
> image "should" be better for a given total acquisition time, because
> a smaller fraction of the total exposure time is spent in retrace
> (about 30% of the time is usually used for retrace in fast scan.
> Ergo, the fraction of the frame time spent actually collecting signal
> is about 70% at 'fast scan" and more like 90% at a 4x slower scan
> rate. However, you seem to know the actual pixel dwell time, so this
> accurate (rather than calculated from other data) then retrace should
> not be a factor.
>
> I haven't read this whole thread but has anyone mentioned the
> electronic bandwidth of the amplifier leading up to the digitizer?
> This should be set to a time constant that is at least 4x slower
> (maybe 5x if we consider the lower proportion of retrace time)? If it
> is not, then any benefit of longer dwell time will be lost (because
> the value of the signal at the instant it is digitized will only be
> characteristic of the shorter, fast scan pixel). To my knowledge only
> BioRad did true box-car averaging where they integrated all the
> current presented during the pixel, no matter how long it took.
>
> As far as vibration or drift(of the stage or the scanning coil
> currents) is concerned, fast scan will cause blur to the whole image,
> while slower scanning will more likely cause distortion. Although
> changing the scan speed by only a factor of 4 (rather than maybe 100
> or even 1,000, as in a SEM) should not show much of this effect.
>
> As far as analog vs, photon counting: In photon counting, the
> bandwidth argument has no validity (assuming that the system merely
> counts the pulses for a longer time as slow scan.) because what is
> important then is the bandwidth up until the counter.
>
> But it is a rare system that can do photon counting at "normal"
> signal levels without losing significant signal to pulse pileup.
> Pileup will tend to clip bright parts of the image, perhaps making
> them look "smoother" .
>
> Finally, what did you all decide you meant by "averaging"? Kalman
> averaging will give similar results (apart from the factors above. A
> running (or exponential) average, will give a factor of at least 2
> less efficient use of the signal (maybe worse if you get into weak
> signals).
>
> You talk about a "camera expert" and "noise suppression", is he
> talking about the tricks used to make pictures made with digital
> cameras look better? That is a whole 'nuther can of worms and needs a
> longer discussion. It should have little bearing on microscopical
> imaging unless you are taking images off your Yokogawa using a Nikon
> D3.
>
> As far as the effect of scan rate on bleaching is concerned, there
> has long been a debate over whether spreading the damage around fast
> perhaps stops the buildup of, say singlet oxygen, to dangerous levels
> in one location. Those scanning at video rate claimed that they could
> watch their specimens longer because of this effect (I guess that the
> assumption was that natural mechanisms for detoxification were
> overwhelmed if the beam sat in one place too long.).
>
> I once tried to  prove this by spending some time at the Noran
> factory, but never got anything definitive. But it could be true,
> because the disk-scanner folk make the same claim with some support.
>
> Jim Pawley
> At the 16th UBC Course.
>
>    
>> To join, leave or search the confocal microscopy listserv, go to:
>> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
>> *****
>>
>> I agree with Julio and Brian about the Zeiss 510 - averaged images were
>> always less noisy than "dwelled" images.  I always taught that point in
>> training sessions and showed side by side comparisons; newbies could
>>      
> clearly
>    
>> see the benefit of averaging over dwelling.  However this isn't the
>>      
> case on
>    
>> my 710 or 700, I see no difference (just by eye!) between averaging and
>> dwelling (~800 volt gain comparing 4-8 averages to dwell times 4-8x
>>      
> slower
>    
>> than whatever max. is [1~3 us]).
>>
>> -Esteban
>>
>>
>> On Thu, Jun 16, 2011 at 2:38 PM, Armstrong, Brian<[hidden email]>
>> wrote:
>>      
>>>   *****
>>>   To join, leave or search the confocal microscopy listserv, go to:
>>>   http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
>>>   *****
>>>
>>>   I have not done a careful analysis of this either, and I am not
>>>        
> quite sure
>    
>> how you would, however I share the viewpoint of Julio exactly,
>>      
> 1.6usec/pix
>    
>> and 2-4 ave.
>>      
>>>
>>>
>>>   Brian Armstrong PhD
>>>   Light Microscopy Core
>>>   Beckman Research Institute
>>>   1450 East Duarte Rd
>>>   Duarte, CA 91010
>>>   626-256-4673 x62872
>>>
>>>        
>> http://www.cityofhope.org/SharedResources/LightMicroscopy/LightMicroHom
>>      
> e.htm
>    
>>>
>>>   -----Original Message-----
>>>   From: Confocal Microscopy List
>>>        
> [mailto:[hidden email]]
>    
>> On Behalf Of Julio Vazquez
>>      
>>>   Sent: Thursday, June 16, 2011 2:21 PM
>>>   To: [hidden email]
>>>   Subject: Re: averaging vs. accumulation for noise reduction - is
>>>        
> there a
>    
>> difference?
>>      
>>>   *****
>>>   To join, leave or search the confocal microscopy listserv, go to:
>>>   http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
>>>   *****
>>>
>>>   This is what I noticed empirically on our Zeiss LSM 510, where
>>>        
> averaging
>    
>> tends to give somewhat better noise reduction than increasing dwell
>>      
> time.
>    
>> Under "normal" imaging conditions, we typically use a dwell time of
>>      
> 1.6-3.2
>    
>> microseconds. Increasing the dwell time to greater than  3.2
>>      
> microseconds
>    
>> tends to result in more bleaching and somewhat reduced signal.
>>      
> Typically, we
>    
>> use 1.6 microseconds dwell time, and 2-4 averages, depending on the
>>      
> sample.
>    
>>>   --
>>>   Julio Vazquez
>>>   Fred Hutchinson Cancer Research Center
>>>   Seattle, WA
>>>
>>>   http://www.fhcrc.org/
>>>
>>>
>>>   On Jun 16, 2011, at 2:08 PM, Moninger, Thomas wrote:
>>>
>>>        
>>>>   Stan,
>>>>
>>>>   I've been told by Carl Z. engineers that in general averaging (I
>>>>          
> usually
>    
>> use line, not frame) tends to yield better S/N then does increasing
>>      
> dwell
>    
>> time. As Lloyd commented this may be model specific. I have not done
>>      
> any
>    
>> analysis to confirm this however....
>>      
>>>>   Tom
>>>>          
>>>
>>>
>>>        
> ---------------------------------------------------------------------
>    
>>>   SECURITY/CONFIDENTIALITY WARNING:
>>>   This message and any attachments are intended solely for the
>>>        
> individual or
>    
>> entity to which they are addressed. This communication may contain
>> information that is privileged, confidential, or exempt from disclosure
>> under applicable law (e.g., personal health information, research data,
>> financial information). Because this e-mail has been sent without
>> encryption, individuals other than the intended recipient may be able
>>      
> to
>    
>> view the information, forward it to others or tamper with the
>>      
> information
>    
>> without the knowledge or consent of the sender. If you are not the
>>      
> intended
>    
>> recipient, or the employee or person responsible for delivering the
>>      
> message
>    
>> to the intended recipient, any dissemination, distribution or copying
>>      
> of the
>    
>> communication is strictly prohibited. If you received the communication
>>      
> in
>    
>> error, please notify the sender immediately by replying to this message
>>      
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>> deleting the message and any accompanying files from your system. If,
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>>>        
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>    
>>>        
>
>    

> example, resonant scans might be digitized at 8-bit for the sake of
> speed, and non-resonant ones at 12 bit.  Brightness is then just a
> function of the display algorithm.
>
>                     Guy
>
>
> Optical Imaging Techniques in Cell Biology
> by Guy Cox    CRC Press / Taylor&  Francis
>       http://www.guycox.com/optical.htm
> ______________________________________________
> Associate Professor Guy Cox, MA, DPhil(Oxon)
> Australian Centre for Microscopy&  Microanalysis,
> Madsen Building F09, University of Sydney, NSW 2006
>
> Phone +61 2 9351 3176     Fax +61 2 9351 7682
>               Mobile 0413 281 861
> ______________________________________________
>        http://www.guycox.net
>
>
>
> -----Original Message-----
> From: Confocal Microscopy List

> difference?
>
> *****
> To join, leave or search the confocal microscopy listserv, go to:
> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> *****
>
> Hi all,
>
> I haven't seen these images but the "dwell" image (slower scan?)
> image "should" be better for a given total acquisition time, because
> a smaller fraction of the total exposure time is spent in retrace
> (about 30% of the time is usually used for retrace in fast scan.
> Ergo, the fraction of the frame time spent actually collecting signal
> is about 70% at 'fast scan" and more like 90% at a 4x slower scan
> rate. However, you seem to know the actual pixel dwell time, so this
> accurate (rather than calculated from other data) then retrace should
> not be a factor.
>
> I haven't read this whole thread but has anyone mentioned the
> electronic bandwidth of the amplifier leading up to the digitizer?
> This should be set to a time constant that is at least 4x slower
> (maybe 5x if we consider the lower proportion of retrace time)? If it
> is not, then any benefit of longer dwell time will be lost (because
> the value of the signal at the instant it is digitized will only be
> characteristic of the shorter, fast scan pixel). To my knowledge only
> BioRad did true box-car averaging where they integrated all the
> current presented during the pixel, no matter how long it took.
>
> As far as vibration or drift(of the stage or the scanning coil
> currents) is concerned, fast scan will cause blur to the whole image,
> while slower scanning will more likely cause distortion. Although
> changing the scan speed by only a factor of 4 (rather than maybe 100
> or even 1,000, as in a SEM) should not show much of this effect.
>
> As far as analog vs, photon counting: In photon counting, the
> bandwidth argument has no validity (assuming that the system merely
> counts the pulses for a longer time as slow scan.) because what is
> important then is the bandwidth up until the counter.
>
> But it is a rare system that can do photon counting at "normal"
> signal levels without losing significant signal to pulse pileup.
> Pileup will tend to clip bright parts of the image, perhaps making
> them look "smoother" .
>
> Finally, what did you all decide you meant by "averaging"? Kalman
> averaging will give similar results (apart from the factors above. A
> running (or exponential) average, will give a factor of at least 2
> less efficient use of the signal (maybe worse if you get into weak
> signals).
>
> You talk about a "camera expert" and "noise suppression", is he
> talking about the tricks used to make pictures made with digital
> cameras look better? That is a whole 'nuther can of worms and needs a
> longer discussion. It should have little bearing on microscopical
> imaging unless you are taking images off your Yokogawa using a Nikon
> D3.
>
> As far as the effect of scan rate on bleaching is concerned, there
> has long been a debate over whether spreading the damage around fast
> perhaps stops the buildup of, say singlet oxygen, to dangerous levels
> in one location. Those scanning at video rate claimed that they could
> watch their specimens longer because of this effect (I guess that the
> assumption was that natural mechanisms for detoxification were
> overwhelmed if the beam sat in one place too long.).
>
> I once tried to  prove this by spending some time at the Noran
> factory, but never got anything definitive. But it could be true,
> because the disk-scanner folk make the same claim with some support.
>
> Jim Pawley
> At the 16th UBC Course.
>
>    
>> To join, leave or search the confocal microscopy listserv, go to:
>> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
>> *****
>>
>> I agree with Julio and Brian about the Zeiss 510 - averaged images

>> dwelling (~800 volt gain comparing 4-8 averages to dwell times 4-8x
>>      
> slower
>    
>> than whatever max. is [1~3 us]).
>>
>> -Esteban
>>
>>
>> On Thu, Jun 16, 2011 at 2:38 PM, Armstrong, Brian<[hidden email]>
>> wrote:
>>      
>>>   *****
>>>   To join, leave or search the confocal microscopy listserv, go to:
>>>   http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
>>>   *****
>>>
>>>   I have not done a careful analysis of this either, and I am not
>>>        
> quite sure
>    
>> how you would, however I share the viewpoint of Julio exactly,
>>      
> 1.6usec/pix
>    
>> and 2-4 ave.
>>      
>>>
>>>
>>>   Brian Armstrong PhD
>>>   Light Microscopy Core
>>>   Beckman Research Institute
>>>   1450 East Duarte Rd
>>>   Duarte, CA 91010
>>>   626-256-4673 x62872
>>>
>>>        
>>

>>      
> e.htm
>    
>>>
>>>   -----Original Message-----
>>>   From: Confocal Microscopy List
>>>        
> [mailto:[hidden email]]
>    
>> On Behalf Of Julio Vazquez
>>      
>>>   Sent: Thursday, June 16, 2011 2:21 PM
>>>   To: [hidden email]
>>>   Subject: Re: averaging vs. accumulation for noise reduction - is
>>>        
> there a
>    
>> difference?
>>      
>>>   *****
>>>   To join, leave or search the confocal microscopy listserv, go to:
>>>   http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
>>>   *****
>>>
>>>   This is what I noticed empirically on our Zeiss LSM 510, where
>>>        
> averaging
>    
>> tends to give somewhat better noise reduction than increasing dwell
>>      
> time.
>    
>> Under "normal" imaging conditions, we typically use a dwell time of
>>      
> 1.6-3.2
>    
>> microseconds. Increasing the dwell time to greater than  3.2
>>      
> microseconds
>    
>> tends to result in more bleaching and somewhat reduced signal.
>>      
> Typically, we
>    
>> use 1.6 microseconds dwell time, and 2-4 averages, depending on the
>>      
> sample.
>    
>>>   --
>>>   Julio Vazquez
>>>   Fred Hutchinson Cancer Research Center
>>>   Seattle, WA
>>>
>>>   http://www.fhcrc.org/
>>>
>>>
>>>   On Jun 16, 2011, at 2:08 PM, Moninger, Thomas wrote:
>>>
>>>        
>>>>   Stan,
>>>>
>>>>   I've been told by Carl Z. engineers that in general averaging (I
>>>>          
> usually
>    
>> use line, not frame) tends to yield better S/N then does increasing
>>      
> dwell
>    
>> time. As Lloyd commented this may be model specific. I have not done
>>      
> any
>    
>> analysis to confirm this however....
>>      
>>>>   Tom
>>>>          
>>>
>>>
>>>        
> ---------------------------------------------------------------------
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>
>Very interesting discussion.
>
>I was just wondering. We talk about S/N. If you acquire a single
>frame for longer I would expect you also accumulate more noise in
>the image, if you average your signal in each image your sample
>should be more or less the same while the noise (random) is
>averaged. So would you not expect a better S/N with averaging when
>all else is equal?
>
>Kees
>
>Senior Experimental Officer
>Centre for Core Biotechnology Services
>University of Leicester, UK
>
>http://www.le.ac.uk/biochem/microscopy/home.html
>
>
>-----Original Message-----
>From: Confocal Microscopy List
>[mailto:[hidden email]] On Behalf Of Stanislav
>Vitha
>Sent: 16 June 2011 17:26
>To: [hidden email]
>Subject: averaging vs. accumulation for noise reduction - is there a
>difference?
>
>*****
>To join, leave or search the confocal microscopy listserv, go to:
>http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
>*****
>
>Hallo,
>this is a very basic question, but I cannot figure this out from what I have
>been reading, so a simple explanation for a non-physicist would be much
>appreciated:
>
>Is there a real difference in the improvement of the signal to noise ratio
>between frame averaging (or accumulation) and longer dwell times (slower
>scan) for a point-scanning confocal witrh a PMT detector?
>
>For instance, using single point scanning confocal, 12-bit acquisition.
>
>a) averaging (or accumulating) 5 frames, 4 microseconds per pixel
>b) acquiring a single frame, 20 microseconds per pixel
>
>Assumptions:
>no saturation of the detector;
>stable environmental conditions, no focus drift, etc
>
>Would it matter (for the dfference between the two scenarios) if it was analog
>detection or photon counting detection?
>
>I will run this little test later, but I am curious what you think.
>
>I thought that at least for the photon counting mode, the two important
>factors would be the dark counts and the total number of counts detected, so
>whether it is acquired in one scan or in 5 scans, it should be the same. My
>camera expert here insists that the averaging scheme will give better noise
>suppression.
>
>Thanks!
>
>
>Stan Vitha
>
>Microscopy and Imaging Center
>Texas A&M University