Posted by
Andreas Bruckbauer on
URL: http://confocal-microscopy-list.275.s1.nabble.com/Basic-live-cell-imaging-question-tp5687698p5710782.html
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Hi John,
I recently tested the Olympus 100x NA 1.65 objective which uses special coverslips and oil with refractive index 1.78 against our 100x NA 1.45 lens. For single molecule TIRF directly at the coverslip i get 2-3 times higher signal with the 1.65 NA lens. This was in good agreement to a calculation based on classical electrodynamics which gave 2.9x more signal in the case of the 1.65 lens. However when i calculted the case for focussing one micron into the cell, the 1.65 lens had a slight disadvantage, more reflection due to the higher difference of refractive indices. This calculation does not account for PSFs or aberations it just deals with plane waves and dipol excitation/emission. However it shows quite clearly that It is really the coupling of the near-field of the oscillating dipol to the propagating waves in the lens which gives rise to increased signal in the high NA case, this does not work if the molecule is more than 1/2 wavelength away from the interface glass/cell.
best wishes
Andreas
-----Original Message-----
From: John Oreopoulos <
[hidden email]>
To:
[hidden email]
Sent: Fri, 5 Nov 2010 18:31
Subject: Re: Basic live cell imaging question...
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Hi Jim,
I'm wondering if you can clear up a few things related to this topic. You said
in your last email that the higher NA rays in a water-glass situation do not get
into the objective, even in the case of TIRF. There is a very nice paper by Jorg
Enderlein's group that uses a very simple technique to measure the actual NA of
an objective which involves viewing the distribution of light rays in the back
focal plane of an objective with the use of a Bertrand lens:
http://www.opticsinfobase.org/oe/abstract.cfm?uri=oe-13-23-9409And another similar paper by Mattheyses and Axelrod:
http://spiedl.aip.org/getabs/servlet/GetabsServlet?prog=normal&id=JBOPFO000010000005054007000001&idtype=cvips&gifs=yes&ref=noBoth of these papers clearly show that a large percentage of the light actually
does propagate into the objective lens beyond the critical angle. However, you
did also allude to "thin aqueous biological" in vitro specimens, the ones that
are typical of single-molecule experiments where the material under
investigation has been separated from the cell, and both of these papers made
their measurements under similar conditions, so maybe this is only a special
case.
My question is, does this situation only occur for fluorescent objects that are
very near the glass-water interface? That is to say, if I were to view a
fluorescent cellular sample the same way (with a Bertrand lens, widefield
illumination, focused slightly into the cell), would I see that most of the
light propagates into the oil immersion objective BELOW the critical angle (and
hence the effective lower NA)?
As for a "quantum mechanical explanation" of why the other situation works, it
seems that Hellen and Axelrod came up with an explanation some time ago that
does not involve quantum mechanics at all, and it can be explained using
classical electrodynamics... but I've had trouble following this paper because
it gets rather complicated with the math:
Hellen, E.H. and D. Axelrod, Fluorescence emission at dielectric and metal-film
interfaces. Journal of the Optical Society of America B-Optical Physics, 1987.
4(3): p. 337-350.
Axelrod, D., Emission of fluorescence at an interface, in Methods in cell
biology, T. Langsing and Y. Wang, Editors. 1989, Academic Press: San Diego. p.
399-416.
There is a very simple diagram in the second book chapter that basically shows
very oblique light rays emitted by a fluorescent molecule near an interface (the
near-field) can turn into propagating evanescent waves that get coupled back
into the higher index medium. This website talks a bit more about this (see
Figure 6):
http://micro.magnet.fsu.edu/primer/techniques/fluorescence/tirf/tirfintro.htmlJohn Oreopoulos
On 2010-11-05, at 11:33 AM, James Pawley wrote:
> *****
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>
>> I always wonder if a water immersion lens is better than an oil immersion
lens for live cell imaging. Both have the wrong RI for cells. Water too low, oil
too high. However, the NA of an oil lens is higher than from a water lens, so
the oil objective should be more light efficient and your resolution should be a
little better. Or am I wrong....?
>>
>> kees
>
>
> Hi Kees,
>
> Yes, I am afraid that you are wrong. The higher NA rays, that an NA 1.4 lens
might accept if it were used with an oiled specimen, are totally reflected at
the water-glass interface and do not get into the objective. Oil lenses work
well for TIRF because the "specimen" is just the thin layer near the interface
in which fluorescence is excited by the evanescent wave. But the cone of light
that actually forms the image (i.e., not counting the part that is probably used
for the high-angle excitation) will still be about NA 1.25.
>
> The other "thin aqueous biological specimens" that were productively viewed
with an oil objective were the various fiber systems (isolated microtubules,
actin filaments etc. lying on a slide, in media) that were visualized using
video-enhanced contrast DIC by Shinya Inoue and Robert Allen back in the early
1980s. Although the exact quantum-mechanical explanation of the interactions
near this specimen is beyond me, it seems likely that these structures were so
close to the glass that they were essentially part of it in terms of maximum
angle at which scattered rays could enter the objective. In any case, the raw
resolution of the recorded images was about that of a normal NA 1.4 objective
with the green light that they used. The ability to visualize much smaller
structures was more a "detection of their presence on a clear background" than a
matter of resolving them.
>
> The rationale for using oil in those days was that there really weren't any
good, high-NA water objectives available. (Here is a good place to reemphasize
Guy's point about the absolute necessity of carefully adjusting the coverslip
correction collar. At NA 1.2, aim for an accuracy of <+/- 2µm of
water-replaced-by glass. This is less important with oil objectives because oil
and coverslip have about the same RI.)
>
> As the RI of water is about 1.33, one might assume that one could use an
objective with an NA of up to 1.33. The reason this doesn't help much is that,
although the rays between 1.2 and 1.33 may not be totally reflected at the
water-glass interface, they are still highly reflected. (Just remember how
bright the image of the sun is when it reflects off a pane of glass at glancing
incidence. Although some sunlight is still being refracted through the glass
into the building, it will be dim because most of the light was reflected.)
>
> And finally, as mentioned by others, there is the matter of spherical
aberration (apparently my favorite topic!). How is this important? If you are
looking at large fluorescent objects (say >1µm), then it isn't quite so
important. Assuming it is not lost to reflection at the glass-water interface, a
larger NA lens will accept more light and if it is not absorbed or reflected
while passing through the optics, this light will end up in the image somewhere
close to its proper location, making the blob appear brighter than it would be
otherwise. However, if you are hoping that the higher NA of the oil lens will
yield better resolution on a water specimen, forget it. As Rimas Juskaitis
makes clear in Chapter 11 of The Handbook, even under optimal conditions (i.e.,
the right oil, temp etc) the best 1.4 objectives then available were only free
from phase error up to NA 1.35 (i.e., the rays between 1.35 and 1.4 were passing
the objective but not being focused properly and hence not contributing the a
reduction in the imaged size of a point object.) I don't know how the newer
1.45, 1.49 and 1.65 objectives would perform under his very stringent test
conditions but I would like to point out that he only got the old ones to work
at 1.35 by controlling the oil temperature to +/- 1deg C.
>
> Once SA is present, the image of a point object gets bigger in a complicated
way (it is hard to define the PSF of an aberrated image with a single number.).
This means not only that the resolution is reduced, but that that the brightest
part of this image will be dimmer than it would have been without the
aberration. i.e. The high-NA oil image of a point object will be dimmer than the
aberration-free image from a water lens with slightly lower "faceplate" NA. The
best plan is to always include small (<.3µm) fluorescent beads in your
preparations and before you start imaging "for real," focus up and down on the
beads "by eye" to make sure that the slightly-out-of-focus image seen above
focus, looks very much like that seen the same amount below focus. If this is
true, then SA should not be a problem.
>
> What I am trying to say is that resolution isn't always proportional to the
number on the side of the objective. Everything else has to be "perfect" and it
seldom is. As you point out, cells are neither water or oil. It is worse than
that. Their internal RI is extremely variable, which is why DIC and phase show
strong contrast of subcellular details.
>
> But that is another story for another hour...
>
> Regards,
>
> Jim Pawley
>
> *********************************************************************************
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223, Zoology Research Building, FAX 608-265-5315
> 1117 Johnson Ave., Madison, WI, 53706
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> "If it ain't diffraction, it must be statistics." Anon.
>
>
>
>
>> -----Original Message-----
>> From: Confocal Microscopy List [mailto:
[hidden email]] On
Behalf Of Gert van Cappellen
>> Sent: 04 November 2010 20:38
>> To:
[hidden email]
>> Subject: Re: Basic live cell imaging question...
>>
>> *****
>> To join, leave or search the confocal microscopy listserv, go to:
>>
http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy>> *****
>>
>> I'm quite sure the cells will also survive an oil immersion lens and
>> normally this gives enough information for single cells. However a water
>> immersion lens is better but certainly not necessary.
>>
>> Best regards,
>> Gert
>>
>> Op 4-11-2010 2:03, Axel Kurt Preuss schreef:
>>> You need a water immersion object or have to build one
>>>
>>>
>>> Cheers
>>>
>>> Axel
>>> -----
>>> Axel K Preuss, PhD,
>>> Central Imaging, IMCB, A*Star, 61 Biopolis Dr, 6-19B, Singapore 138673,
sent from 9271.5622
>>>
>>>
>>> On Nov 4, 2010, at 4:06 AM, Gert van Cappellen<
[hidden email]>
wrote:
>>>
>>>> *****
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>>>>
>>>> Culture your cells on a round coverslip. Take an object glas glue a
>>>> square piece of non-toxic rubber with a round hole on it. Fill this with
>>>> CO2 satured medium somewaht more as the volume of the hole. Put your
>>>> coverslip on it, with the cells to the medium off course. Press it
>>>> gently down and the glass will seal itself to the rubber ring. Now your
>>>> cells will survive for a couple of hours, so you can do the first
>>>> imaging. For real experiments you have to find a way to heat the object
>>>> glass to 37C.
>>>>
>>>> Good luck, Gert
>>>>
>>>> Op 29-10-2010 21:00, Dolphin, Colin schreef:
>>>>> *****
>>>>> To join, leave or search the confocal microscopy listserv, go to:
>>>>>
http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy>>>>> *****
>>>>>
>>>>> We would like to do live cell imaging - mammalian cell lines - but only
have direct access to an upright Olympus BX61. We don't really need complicated
perfusion chambers, etc just something simple. We're real neophytes so all
suggestions gratefully received.
>>>>>
>>>>> Colin
>>>>>
>>> Note: This message may contain confidential information. If this Email/Fax
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>
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