TREA

Optical near-field microscope

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Information

  • Patent Grant
  • 6674057
  • Patent Number
    6,674,057
  • Date Filed
    Thursday, May 4, 2000
    24 years ago
  • Date Issued
    Tuesday, January 6, 2004
    21 years ago
Information
Abstract
Near-field optical microscope with a probe tip which is arranged on one side of a light-transmitting specimen and moved in a scanning manner. The probe tip serves as a point light source. Optics for collecting light transmitted through the specimen and transmitting it to a detection unit or for collecting illumination light are provided on the other side of the specimen. The movement of the probe tip is adapted to on the detection side, or the probe serves to detect specimen light. A detection unit is arranged following the probe in the direction of illumination, and a scanning illumination adapted to the probe movement is carried out on the other side of the specimen.
Description




BACKGROUND OF THE INVENTION




a) Field of the Invention




The invention relates to an improvement in optical near-field microscopes.




b) Description of Related Art





FIG. 1

shows the well-known construction of a SNOM arrangement. A near-field probe shaped as a tip SP is located at a distance of less than the light wavelength above the surface of a transparent specimen P. The specimen is held on a scanning table STI which is movable in the X/Y/z direction, so that the specimen can be scanned linewise by the tip SP. The scanning table STI is controlled by a control unit AE. The light which is not absorbed is collected by an objective O


1


and its intensity is measured by a detector DT, for example, an avalanche diode or a PMT, arranged behind a pinhole PH for suppressing scattered light. An image of the surface of the specimen is composed from this. It is further known to reverse the light path and illuminate the specimen through the objective, the transmitted light being collected through the tip SP.




The scanning movement of the specimen results in restrictions in the specimen geometry and in the maximum attainable scanning speed. One reason against a scanning movement of the tip is that the probe and optical construction move relative to one another. Accordingly, it is not possible, for example, to detect the light emitted by the probe confocally or to illuminate confocally the specimen site under examination. The first arrangement is advantageous for suppression of scattered light, the second arrangement prevents bleaching out of dyes in fluorescence measurements. Moreover, it is not possible to stop down larger or smaller apertures (e.g., forbidden light).




OBJECT AND SUMMARY OF THE INVENTION




It is the primary object of the invention to avoid these disadvantages. This object is met by a near-field optical microscope according to the invention, with a probe tip which is arranged on one side of a light transmitting specimen and moved in a scanning manner. The probe tip serves as a point light source, wherein optics for collecting light transmitted through the specimen and transmitting it to a detection unit or for collecting illumination light are provided on the other side of the specimen. The movement of the probe tip is adapted to on the detection side.











Preferred further developments are contained in the dependent claims. The invention will be explained more fully with reference to the schematic drawings.




BRIEF DESCRIPTION OF THE DRAWINGS





FIG. 1

shows the well-known construction of a SNOM arrangement as described above;





FIG. 2

shows a first optical arrangement with the probe as light source;





FIG. 3

shows another construction;





FIG. 4

shows another construction;





FIG. 5

shows the moving probe tip in an inverse microscope beam path of a laser scanning microscope; and





FIG. 6

shows the moving probe tip for detection with an LSM beam path for specimen illumination.











DESCRIPTION OF THE PREFERRED EMBODIMENTS





FIG. 2

shows an arrangement according to the invention in which the probe SP is mounted in a scanning unit STI


1


, for example, a piezo scanner, and carries out a scanning movement. The instantaneous position of the probe SP is detected via a path measuring system WM and the pinhole PH is correspondingly tracked by means of a scanning unit STI


2


. If the detector DT has a sufficiently large sensitive surface, it need not be moved; otherwise, it can be moved jointly with the pinhole PH by STI


2


.




The path measuring system WM and the scanning unit STI


2


are connected with the control unit AE.




In

FIG. 3

, instead of a tracking of the pinhole PH, the control of a scanning mirror SM arranged downstream of the objective O


1


is carried out, this scanning mirror SM being controlled via the control unit AE corresponding to the movement of the tip SP in such a way that the tip of the probe SP is always imaged on the pinhole PH.




The light path can be reversed in the embodiment forms shown in

FIGS. 2 and 3

. The probe tip is illuminated confocally and the light collected by the probe is supplied to the detector.




The construction realized in

FIG. 4

makes do on the detection side without moving parts. The individual pixels of a CCD camera take over the function of the confocal pinhole. The path measuring system WM and control unit AE ensure that only the confocally illuminated pixels are active.




In

FIGS. 5 and 6

, the near-field optical microscope SNOM is arranged above the object table of an inverse light microscope M. The scanning module S of a confocal laser scanning microscope (LSM), or parts thereof, is located at this light microscope.




A laser module LM contains laser L for illuminating the specimen P via light-conducting fibers LF


1


, LF


2


.




The lasers are combined via splitter mirrors TS and are coupled into the light-conducting fibers LF


1


,


2


via an AOTF and an input-coupling unit EO. The scan head S can be attached to the phototube of an upright microscope as well as to a side output of an inverse microscope M as is shown.




The microscope beam path in the microscope unit M comprises a light source Q, illumination optics O


2


, beam splitter ST


1


, objective O


3


, specimen P and, in the direction of observation/detection, a first tube lens TL


1


, an observation beam path with a second tube lens TL


2


and a beam splitter ST for coupling in and coupling out the scanning beam.




The light from the laser L is coupled into the tip SP of the SNOM in FIG.


5


. The actual scanning unit S comprises a scanning objective SL, scanner SC with scanning mirrors, not shown, deflection mirror SP, and shared imaging optics O


4


for the detection channels.




The deflection mirror SP arranged following the imaging optics O


4


reflects the radiation coming from the specimen P in the direction of dichroic beam splitters DS


1


-


3


in the convergent beam path of the imaging optics O


4


, wherein pinholes PH


1


-


4


which are displaceable in the direction of and perpendicular to the optical axis and which are adjustable in diameter are arranged along with emission filters and suitable receiver elements individually for each detection channel following the beam splitters DS


1


-


3


.




The current position of the tip SP is again determined via the path measuring system WM and is controlled via the control unit AE of the scanning mirror SC of the LSM scanning module S in such a way that the tip SP is imaged on the pinholes PH


1


-


4


.




In

FIG. 6

, the transmitted light is detected by the tip SP and a detector DT. The illumination or fluorescence excitation is carried out by the confocal illumination beam path of the LSM scan module S.




Coupling into the light-conducting fibers LF


1


, LF


2


is carried out by means of displaceable collimating optics KO and beam deflecting elements ST


2


.




A monitoring beam path is stopped down by means of a partially transmitting mirror ST


3


in the direction of a monitor diode MD, in front of which line filters LF and neutral filters ND are advantageously arranged on a rotatable filter wheel, not shown.




The illumination spot tracks the movement of the tip over STI


1


by means of the scanning mirror SC, the path measuring system WM and the control unit AE.




While the foregoing description and drawings represent the present invention, it will be obvious to those skilled in the art that various changes may be made therein without departing from the true spirit and scope of the present invention.



Claims
  • 1. A near-field optical microscope comprising:a probe tip which is arranged on one side of a light-transmitting specimen and moved in a scanning manner, said probe tip serving as a point light source; optics for collecting light transmitted through the specimen and transmitting it to a detection unit or for collecting illumination light being provided on the other side of the specimen, wherein the movement of the probe tip is adapted to on the detection side; and wherein the probe tip is a point light source and a control unit is provided for synchronizing scanning tracking of a detection unit beam path with the movement of the probe tip; wherein a scanning unit is arranged downstream in the detection beam path and images the illumination light on a detector or a pinhole arranged in front of a detector by means of synchronized control; and wherein the scanning unit is a scanning mirror of a laser scanning microscope.
  • 2. The near-field optical microscope according to claim 1, wherein a tracked beam path images the probe on the detector confocally.
  • 3. The near-field optical microscope according to claim 1, wherein the detection unit is tracked.
  • 4. The near-field optical microscope according to claim 1, wherein a detector with a pinhole arranged in front of it is tracked.
  • 5. The near-field optical microscope according to claim 1, wherein the detection unit is realized over a surface area and a synchronized tracking of a pinhole arranged in front of the detection unit is carried out.
  • 6. The near-field optical microscope according to claim 1, wherein the probe is imaged on a detector comprising a plurality of elements and the readout of the individual elements is synchronized with the scanning movement of the probe.
  • 7. The near-field optical microscope according to claim 6, wherein the imaging of the probe on the detector includes the use of a CCD camera.
  • 8. The near-field optical microscope according to claim 6, wherein the quantity of simultaneously active elements is only that quantity sufficient to ensure a confocal imaging.
  • 9. The near-field optical microscope according to claim 1, wherein the near-field probe is arranged in the beam path of a microscope on the side opposite to the microscope objective.
  • 10. The near-field optical microscope according to claim 1, wherein the microscope has a lateral coupling in of a scanning beam path.
Priority Claims (1)
Number Date Country Kind
198 22 869 May 1998 DE
PCT Information
Filing Document Filing Date Country Kind
PCT/EP99/03425 WO 00
Publishing Document Publishing Date Country Kind
WO99/61949 12/2/1999 WO A
US Referenced Citations (6)
Number Name Date Kind
5138159 Takase et al. Aug 1992 A
5304795 Fujihira et al. Apr 1994 A
5333495 Yamaguchi et al. Aug 1994 A
5343460 Miyazaki et al. Aug 1994 A
5361314 Kopelman et al. Nov 1994 A
6229609 Muramatsu et al. May 2001 B1
Foreign Referenced Citations (1)
Number Date Country
WO 9730366 Aug 1997 WO
Non-Patent Literature Citations (2)
Entry
XP 000518228 / Optical Engineering, Aug. 1994 “Super-resolution imaging and detection of fluorescence from single molecules by scanning near-field optical microscopy” Alfred J. Meixner, et al. (pp. 2324-2332).
XP 00511233 / Review of Scientific Instruments, Jun. 1995 “Design and construction of a versatile scanning near-field optical microscope for fluorescence imaging of single molecules” G. Tarrach, et al. (pp. 3569-3575).