fast confocal imaging -- old vs. new technologies

Dear Charu,

Two articles (of mine) address rapid calcium imaging:
2003: illustrates the spatial-temporal limits of calcium imaging
   achieved with single-point/line scanning confocal.
2008: review discusses some tradeoffs and shows an example
    where spinning disk was used to get an areal-view and then
    single-line scanning to obtain highest temporal resolution.
[PDFs of both articles can be found on the last page of my
ed-tech web site www.digital-maze.com; bottom link on left
side navigation bar titled: O'Malley PDFs].
 
In my 2008 review I have unfortunately not included other
newer technologies available only because I had not then
been able to find any highest end spatial-temporal resolution
images published using any of them.  But the bottom
line from a neurobiology perspective is that one can often
use slower frame-scan imaging to determine a location for
single-line scanning to be applied and then the good old
fashioned line-scan still seems to provide the most sensitive and
durable highest-end combined spatial-temporal resolution images
(on the order of 2 msec x microns-squared "dynamic units").
One caveat is that much of the best work has been done by
folks using 2-photon single-line scanning instruments (see
citations in 2008 review).
 
The issue is not how fast can you acquire, but how fast can
you resolve subcellular dynamic events in both space and time.
Acquiring fast and binning over time adds nothing to temporal
resolution.  Figure 3 in my 2003 review illustrates diffusion
of calcium across the plasma membrane and across the nuclear
envelope, acquired with an MRC600 single-line scanner.  My
2008 review covers what I had found thru about late-2007 and
I was not then aware of any spatial-temporal dynamic imaging
results that exceeded the performance of the venerable MRC600
linescan (if there are any older examples that I have missed --
my apologies!).  By trading away some spatial resolution with
a partially opened aperture one can enormously increase signal
throughput allowing one to reduce excitation intensity-- good old
confocal is very good for live cell and live animal imaging.
 
The lack of a continuously-variable aperture on spinning disk
confocals is a serious limitation, but one that might be corrected
by having a set of disks that trade off spatial resolution for greatly
increased signal.  If anyone knows of this being implemented and
used to obtain highest-end dynamic units (for calcium flux, dextran
diffusion, organelle movement, etc.), I am sure that many on the
list would like to see published results--ditto for any such results
with the resonant scanners.  [I have not researched this since 2007,
sorry].  In the example in my 2008 review, a Nipkow disk obtained
nice 2D images at 17 msec intervals (which with 1 um**2 spatial
resolution would yield a dynamic resolution of 17 msec-um**2)
after which 2 msec linescans were then used to explore the finest
temporal structure of calcium sparks (Fig. 2); this was reprinted
work from Lothar Blatter's lab from 2001.
 
My 2008 review discusses some trade offs and issues encountered in fast
imaging, and again my apologies for anything that I have missed.
 
Happy 2010,
Don
 
Don O'Malley
Dept. Biology
[hidden email]
617-373-2284

 

Dear Donald This is what i was exactly looking for.THANK YOU VERY MUCH. I will hold on to your reviews, they seem to be very informative. I will also try finding some published data from these resonant scanners/tandem scanners etc. Great. Thanks and regards CHARU TANWAR Imaging Specialist Advanced Instrumentation Research Facility Jawaharlal Nehru University New Delhi 110067 India. --- On Wed, 6/1/10, O'Malley, Donald <[hidden email]> wrote: From: O'Malley, Donald <[hidden email]> Subject: fast confocal imaging -- old vs. new technologies To: [hidden email] Date: Wednesday, 6 January, 2010, 2:30 PM Dear Charu, Two articles (of mine) address rapid calcium imaging: 2003: illustrates the spatial-temporal limits of calcium imaging    achieved with single-point/line scanning confocal. 2008: review discusses some tradeoffs and shows an example     where spinning disk was used to get an areal-view and then     single-line scanning to obtain highest temporal resolution. [PDFs of both articles can be found on the last page of my ed-tech web site www.digital-maze.com; bottom link on left side navigation bar titled: O'Malley PDFs]. In my 2008 review I have unfortunately not included other newer technologies available only because I had not then been able to find any highest end spatial-temporal resolution images published using any of them.  But the bottom line from a neurobiology perspective is that one can often use slower frame-scan imaging to determine a location for single-line scanning to be applied and then the good old fashioned line-scan still seems to provide the most sensitive and durable highest-end combined spatial-temporal resolution images (on the order of 2 msec x microns-squared "dynamic units"). One caveat is that much of the best work has been done by folks using 2-photon single-line scanning instruments (see citations in 2008 review). The issue is not how fast can you acquire, but how fast can you resolve subcellular dynamic events in both space and time. Acquiring fast and binning over time adds nothing to temporal resolution.  Figure 3 in my 2003 review illustrates diffusion of calcium across the plasma membrane and across the nuclear envelope, acquired with an MRC600 single-line scanner.  My 2008 review covers what I had found thru about late-2007 and I was not then aware of any spatial-temporal dynamic imaging results that exceeded the performance of the venerable MRC600 linescan (if there are any older examples that I have missed -- my apologies!).  By trading away some spatial resolution with a partially opened aperture one can enormously increase signal throughput allowing one to reduce excitation intensity-- good old confocal is very good for live cell and live animal imaging. The lack of a continuously-variable aperture on spinning disk confocals is a serious limitation, but one that might be corrected by having a set of disks that trade off spatial resolution for greatly increased signal.  If anyone knows of this being implemented and used to obtain highest-end dynamic units (for calcium flux, dextran diffusion, organelle movement, etc.), I am sure that many on the list would like to see published results--ditto for any such results with the resonant scanners.  [I have not researched this since 2007, sorry].  In the example in my 2008 review, a Nipkow disk obtained nice 2D images at 17 msec intervals (which with 1 um**2 spatial resolution would yield a dynamic resolution of 17 msec-um**2) after which 2 msec linescans were then used to explore the finest temporal structure of calcium sparks (Fig. 2); this was reprinted work from Lothar Blatter's lab from 2001. My 2008 review discusses some trade offs and issues encountered in fast imaging, and again my apologies for anything that I have missed. Happy 2010, Don Don O'Malley Dept. Biology d.omalley@... 617-373-2284

---

The INTERNET now has a personality. YOURS! See your Yahoo! Homepage.

I am interested on FRAP and photoactivation in wide field microscopes or fast confocal systems such as spinning disk or array scanning systems used in the study of live cells.

Is anybody familiar with the Mosaic Digital Illumination Systems?

http://www.photonic-instruments.com/MicroPoint_Mosaic.aspx

Sounds really cool, but is quite expensive. I would appreciate any input regarding experiences with this equipemnt for the above applications.

We work with live cells in a multiuser core, so we are planning to setup a fast imaging system and would like to be able to perform FRAP and PA applications. The time course of the events studied will range widely from minutes to seconds and perhaps fractions of a second.

Leoncio Vergara MD
Assistant Director
Center for Biomedical Engineering
University of Texas Medical Branch.
Galveston, Texas

Hi Leoncio,

We have two systems that we use for FRAP and photoactivation - a
DeltaVision system with the QLM laser module, and a Yokagawa-type
spinning disk system fitted with the Photonics Digital Mosaic operated
under MetaMorph software.  Both systems work really nicely for both
purposes.  The DeltaVision system, which just targets a single point at
a time, gives faster bleaching or activation, but the Mosaic is really
cool for the region of interest targeting if speed is less of an issue.  
So I think your decision may depend on how often you need to be able to
both bleach and switch to imaging in under a second, as well as on the
optimal type of imaging afterwards (i.e. confocal or widefield).  Like
you, we are operating a core facility and have a wide range of users and
applications on these systems, so rather than going into any more
specific details here, please feel free to contact me offline or give me
a call to discuss your questions in more detail?  I can provide some
absolute bleaching times from comparisons of the same experiment
performed using the two systems, but am reluctant to post them to the
whole world because they were not collected using the most recent
hardware and therefore might be misleading as to the current equipment
capabilities.

All the best - and Happy New Year everybody!
Alison


Vergara, Leoncio A. wrote:
--
Alison J. North, Ph.D.,
Research Assistant Professor and
Director of the Bio-Imaging Resource Center,
The Rockefeller University,
1230 York Avenue,
New York,
NY 10065.
Tel: office ++ 212 327 7488
Tel: lab     ++ 212 327 7486
Fax:         ++ 212 327 7489

Hello Leoncio

We work with live cells in a multi-user core facility as well, and we use the Carl Zeiss LSM 5 Live Duoscan system for our FRAP and PA experiments.  The system gives you a lot of control over the bleaching process and it is very versatile.  Speed is also not an issue with this system, it is quite fast.  It is a line scanning confocal system, so both bleaching and acquisition can be done in fractions of seconds, depending on the settings of your experiment.  If you need any specific information, feel free to contact me directly at [hidden email]

best wishes,

Yevgeniy

________________________________________
From: Confocal Microscopy List [[hidden email]] On Behalf Of Vergara, Leoncio A. [[hidden email]]
Sent: Wednesday, January 06, 2010 6:45 PM
To: [hidden email]
Subject: FRAP and fast confocals and wide field systems

I am interested on FRAP and photoactivation in wide field microscopes or fast confocal systems such as spinning disk or array scanning systems used in the study of live cells.

Is anybody familiar with the Mosaic Digital Illumination Systems?

http://www.photonic-instruments.com/MicroPoint_Mosaic.aspx

Sounds really cool, but is quite expensive. I would appreciate any input regarding experiences with this equipemnt for the above applications.

We work with live cells in a multiuser core, so we are planning to setup a fast imaging system and would like to be able to perform FRAP and PA applications. The time course of the events studied will range widely from minutes to seconds and perhaps fractions of a second.

Leoncio Vergara MD
Assistant Director
Center for Biomedical Engineering
University of Texas Medical Branch.
Galveston, Texas
 
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Dear Leoncio,

Thanks for the reference to this instrument.

Although I have no experience using it, the system seems to use a
computer controlled digital mirror array device (DMD) placed in an
image plane of a laser-based, microscope epi-illumination system.
Turning a micro-mirror "on" produces a diffraction-limited spot of
light in the imaged plane.

The advantage of such a system is its flexibility in being able to
expose the specimen to an "activation" beam" having an arbitrary 2D
shape.* The disadvantage is that laser light that impinges on (the
vast majority?) of the micro-mirrors that are turned "off", is lost.
Assuming that this wasted light it sent to a well-engineered beam
dump, this just means that one needs a (much?) larger laser to do a
certain amount of damage. How much larger depends on the fraction of
your field-of-view you customarily bleach (and on whether an
alternative, single-beam bleach system bleaches in a raster pattern
or by "beam steering").

Another consideration for DMD systems is the stray light that
diffracts off the corners of the mirrors and their surroundings.
Taking the listed contrast ratio of 1,000:1 and assuming that the
chip is a 1,024x768 array, then if only one pixel is turned on, this
beam will constitute only 1.27 ppm of the light striking the chip
while the "stray" light will constitute 1,000 ppm, or about 790x more
light. Clearly, you will have to turn on about 790 bright pixels
before the photons in the intentional pattern equals those in the
stray light striking the rest of the field of view. (These numbers
are approximate as I suspect that the 1,000:1 contrast figure given
is for the DMD device itself and hidden in this specification are
assumptions about the acceptance angle of the following optical
system that may be more appropriate to the optics of a digital
projector than to that of a microscope illumination system. But these
are still matters that should be kept in mind. How much of the
"activation" light strikes the specimen when all the mirror are
turned off?)

More to the point, many of the techniques you mention involve
photochemical processes that may involve intermediates that may
diffuse some distance from the point where the excitation photon was
absorbed. If this is true, one might be interested to know to
accurately one needs to specify the pattern of excitation light.

For instance, at the power levels "normally" used for bleaching in
oxygenated, living cells (bleaching in less than a second, but not in
a ms, and probably using continuous rather than pulsed lasers), most
bleaching is not caused directly by the absorption of a photon so
much as the transfer of the excitation energy to nearby molecules
eventually creating one of a number of excited oxygen species. These
excited molecules can diffuse on the order of micrometers before
reacting. Only some of these reactions are those that cause the
fluorescent molecules to cease fluorescing. Others may interfere with
the very system you want to analyse.

Bleaching at higher power levels (for instance those likely to be
provided by a single, diffraction-limited mW beam) may result in
singlet-state saturation effects whereby an already-excited molecule
absorbs a second photon, perhaps leading to its disintegration
without the need for excited oxygen intermediates.

Alternatively, some "photodamage systems" utilize pulsed lasers.
Pulsed lasers generate peak powers that are 10,000x to 1,000,000x
more intense than those produced by continuous lasers of the same
average power. The photodamage produced at these power levels can be
very different from that produced at lower levels. For instance, the
electronic field vector can become strong enough to produce
electrical breakdown: (micro lightening?) in which case the resulting
damage is not due to (or dependent on) the absorption of the
excitation light by a dye molecule. Such systems are often used to
make holes in cell membranes, or for other types of microsurgery.

I mention this because in other parts of the Photonics www site they
do seem to describe pulsed laser ablation systems of this type.

Photodamage and microsurgery is discussed at much greater length in
Chapters 38 and 39 of The Handbook.

Cheers,

Jim Pawley

* Although this setup can also be used to provide the patterned
illumination used in one type of 3D imaging, I have not discussed
this here, as it seemed that FRAP and PA were the main interests.


               **********************************************
Prof. James B. Pawley,                          Ph.  608-263-3147
Room 223, Zoology Research Building,              
FAX  608-265-5315
1117 Johnson Ave., Madison, WI, 53706  
[hidden email]
3D Microscopy of Living Cells Course, June 12-24, 2010, UBC, Vancouver Canada
Info: http://www.3dcourse.ubc.ca/             Applications due by March 15, 2010
               "If it ain't diffraction, it must be statistics." Anon.

--
               **********************************************
Prof. James B. Pawley,                          Ph.  608-263-3147
Room 223, Zoology Research Building,              
FAX  608-265-5315
1117 Johnson Ave., Madison, WI, 53706  
[hidden email]
3D Microscopy of Living Cells Course, June 12-24, 2010, UBC, Vancouver Canada
Info: http://www.3dcourse.ubc.ca/             Applications due by March 15, 2010
               "If it ain't diffraction, it must be statistics." Anon.