EP2517064A2 - Beleuchtungsverfahren und systeme zur verbesserung der bildauflösung von bildgebungssystemen - Google Patents

Beleuchtungsverfahren und systeme zur verbesserung der bildauflösung von bildgebungssystemen

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Publication number
EP2517064A2
EP2517064A2 EP10843550A EP10843550A EP2517064A2 EP 2517064 A2 EP2517064 A2 EP 2517064A2 EP 10843550 A EP10843550 A EP 10843550A EP 10843550 A EP10843550 A EP 10843550A EP 2517064 A2 EP2517064 A2 EP 2517064A2
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EP
European Patent Office
Prior art keywords
illumination
imaging system
illumination beam
light
region
Prior art date
Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
Withdrawn
Application number
EP10843550A
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English (en)
French (fr)
Inventor
Miao Zhang
Hui Hu
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Individual
Original Assignee
Individual
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Filing date
Publication date
Application filed by Individual filed Critical Individual
Publication of EP2517064A2 publication Critical patent/EP2517064A2/de
Withdrawn legal-status Critical Current

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Classifications

    • GPHYSICS
    • G02OPTICS
    • G02BOPTICAL ELEMENTS, SYSTEMS OR APPARATUS
    • G02B21/00Microscopes
    • G02B21/06Means for illuminating specimens
    • G02B21/08Condensers
    • G02B21/10Condensers affording dark-field illumination
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61BDIAGNOSIS; SURGERY; IDENTIFICATION
    • A61B5/00Measuring for diagnostic purposes; Identification of persons
    • A61B5/0059Measuring for diagnostic purposes; Identification of persons using light, e.g. diagnosis by transillumination, diascopy, fluorescence

Definitions

  • This invention relates to illumination methods and systems for improving image resolution and reducing image noises in imaging systems, and, more particularly, to illumination methods and systems for improving resolution and reducing noises of microscopes in in-vivo, high-resolution or real-time applications.
  • electromagnetic wave such as visible light or ultrasonic wave
  • the electromagnetic wave also referred to light
  • the electromagnetic wave will be interacted with the object.
  • an object such as a tissue
  • a chain of interactions between light and the tissue occurs. These interactions include reflection, refraction, scattering, diffusion, diffraction, etc., all of which change the light path (i.e., redirection) and other light properties (e.g., intensity, phase, and polarization).
  • the interactions also include absorption, which causes light to be attenuated.
  • trans -illumination where the illumination light illuminates the object from one side and the imaging detection system such as objective lens of microscope is positioned on the opposite side of the object to detect the light that passes through the object.
  • the other illumination method is called reflection illumination (also called epi-illumination), where the illumination light illuminates the object from the same side of the imaging detection system such as objective lens and the imaging detection system detects light redirected (e.g., reflected or scattered) backwards by the object.
  • reflection illumination also called epi-illumination
  • the trans -illumination method though used to study a transparent or thin specimen, is not suitable for observing structures underneath opaque thick tissues because light cannot pass through them.
  • the reflection illumination (epi-illumination) method becomes the only feasible option.
  • Microscopic study of in-vivo targets, such as micro vascular structures, underneath tissues poses a severe low-signal, high-noise challenge.
  • the target region of the imaging system is usually at a certain depth underneath the tissue surface. As the observation depth increases, less and less illumination light can reach and interact with the target region to form the useful signals. Moreover, these useful signals are more and more likely to be further absorbed or redirected, without being detected by the imaging system.
  • the intensity of the useful signals detected by imaging system becomes extremely small so that they are buried by the unrelated signals, also called noises, generated outside the target region, and the resulted images are too blurry and noisy to be useful.
  • reducing noises is desired for the improvement of image quality of an imaging system such as intravital microscopy.
  • a reflection illumination method for an imaging system comprises illuminating an object including at least one target region with at least one illumination beam; detecting light redirected by the object from a detectable region of the imaging system; wherein the at least one illumination beam is focused such that the size of a projected illumination beam spot at the target region is reduced.
  • the noises detected by the imaging system can be reduced, and therefore improving image sharpness and the signal-to-noise ratio.
  • the illumination beam is focused by an objective lens of the imaging system.
  • the objective lens is used to focus both the illumination beam and detected light redirected.
  • the projected size of the illumination beam spot at the target region may be less than a half size of the field of view of the imaging system.
  • a method for illumination in an imaging system comprises illuminating an object including at least one target region with at least one illumination beam; detecting light redirected by the object from a detectable region of the imaging system; wherein at least one illumination beam is aimed such that the portion of the detectable region that is under direct illumination is reduced.
  • the portion of the detectable region that is under direct illumination is reduced by controlling one or more of parameters including an oblique angle of the illumination beam, the displacement of the projected illumination beam spot relative to the target region, and, a size of the projected illumination beam spot relative to the target region.
  • the illumination beam is aimed such that the projected illumination beam spot is projected off the center of the field of view of the image system.
  • the portion of the detectable region that is under direct illumination is less than 50% of the total detectable region of the imaging system.
  • the method of reducing direct illumination of the unrelated regions in the detectable region of the imaging system and pin-point focusing illumination beams are combined to achieve the benefits of both.
  • reducing direct illumination of the unrelated regions is achieved by adjusting aiming parameters of the light beams on the object.
  • aiming parameters of the illumination beam include: (1) the oblique angle of the illumination beam; (2) the displacements of the projected beam spot relative to the target region and (3) the size of the projected beam spot relative to the target region.
  • the other parameters include wavelength, intensity, phase, and polarization of the illumination beam.
  • an imaging system comprising an illumination system including at least one illumination beam of light illuming a object including a target region; a detection system for detecting redirected light by the object from a detectable region of the imaging system; and a beam controller for directing the path of the illumination beam of light; wherein the illumination beam of light is such arranged that the overlap of the path of the illumination beam of light and the detectable region is reduced.
  • the beam controller is adjustable by a user by selecting one or more of illumination parameters including an oblique angle of the illumination beam, a displacement of the projected illumination beam spot relative to the target region, and a size of the projected illumination beam spot relative to the target region.
  • the illumination system is configured to project an illumination beam spot off the center of the field of view of the imaging system.
  • the illumination system is configured to project the illumination beam spot outside the field of view of the imaging system.
  • the illumination beam of light is provided from inside a housing of the detection system of the imaging system.
  • the illumination and detection systems share a light directing device.
  • a method is provide to reduce the redirected light, including reflected as well as scattered and other, from being generated by the unrelated regions in the detectable region of the imaging system.
  • a system is provided to distinguish the region of the field of view from the region of the projected beam spot.
  • the projected beam spot is operated primarily off the center of the field of view and can be adjusted by users.
  • image resolution can be improved by reducing or avoiding direct illumination of unrelated regions, particularly in the detectable region of the imaging system.
  • the principles of the present invention can be used in the imaging systems consisting of illumination and detection systems. Examples of such a system include microscope and medical ultrasound scanning.
  • Figure 1 is a schematic block diagram showing an embodiment of the microscopic system according to the principles of the invention.
  • Figure 2 shows the concept of the detectable region of the imaging system, using a schematic view of the Cone Of detected Light (COL) of an exemplary microscopic system, to illustrate one principle of the invention.
  • COL Cone Of detected Light
  • Figure 3A and 3B show a schematic view of how the illumination beam overlaps with the detectable region in prior art intravital microscopy systems.
  • Figure 4 shows a schematic view of the Off-COL Side Illumination, which is an embodiment of the present invention.
  • Figure 5 shows a schematic view of the Pinpoint Illumination, which is an embodiment of the present invention. It shows a case of the Pinpoint Illumination that is called the Pinpoint Off-COL Side Illumination, which is another embodiment of the present invention.
  • Figure 6 shows a schematic view of adjusting the aiming parameters of the illumination beam by users, which is an embodiment of the present invention.
  • Figure 7 is a schematic illustration showing an embodiment of the present invention that implements several embodiments of the present invention shown in Figures 4-6.
  • FIG. 1 shows a block diagram of an embodiment of the imaging system according to the principles of the invention.
  • the imaging system such as a microscopic system 10 use imaging methods 20 including illumination methods and detection methods. It has an illumination system 30 to illuminate light or electromagnetic wave in general onto an object or a target 50 to be studied.
  • the object 50 for example, can be a tissue under investigation.
  • the object 50 include the target region of study 309. The region inside the object but outside the target region 309 is called unrelated regions of study.
  • It also has a detection system 40 to detect redirected light from the object 50.
  • the microscopic imaging methods 20 that can be used on this system include, but are not limited to, the optical microscope, the Fluorescence Microscope, the OPS Microscope and the Confocal Microscope.
  • Figure 2 shows the new concept of the detectable region of the imaging system, using an exemplary microscopic system to illustrate one principle of the invention.
  • the detectable region 301 of the imaging system 10 such as a cone of detected light (COL) of the microscope.
  • the Field Of View (FOV) 302 of the imaging system 10 is the cross-section of the target region 309.
  • the imaging aperture 303 of the imaging system 10 is the opening of the imaging system 10 that determines the amount of the light to be captured in the resulted images.
  • the detectable region of the imaging system 301 is enclosed by the FOV 302 as the apex and the imaging aperture 303 as the base.
  • the detectable region 301 can be in other forms of space such as a hollow rectangular cuboid.
  • the detectable region 301 can be in other forms of space such as a hollow rectangular cuboid.
  • An objective of this disclosure is to design an illumination path inside the tissue relative to the detectable region 301 and FOV 302 to reduce background noises, and, therefore to increase the ratio of intensities of signals versus background noises.
  • the amount of light redirected by each point in the tissue is proportional to the intensity of illumination light impinging upon that point.
  • those points in the direct illumination paths are the primary light redirecting sources. If unrelated regions are directly illuminated, they become the primary noise-generating sources. Furthermore, if those unrelated regions right in front of the imaging detection system, i.e., inside the detectable region 301, are directly illuminated, the noises they generate are most likely to be detected by the imaging system.
  • An aspect of this invention is to reduce the background noises by reducing the direct illumination of unrelated regions, particularly in the detectable region 301 of the imaging system.
  • Direct illumination of a region means the region is directly in the primary illumination beam path.
  • the focal plane and focal distance (also called the working distance) of the imaging system such as objective lens is denoted as 304 and 305, respectively.
  • the axis of the imaging system such as imaging system is denoted as 306.
  • the detectable region 301 represents the region above the target region 309 that is directly under the imaging system. Thus, the light redirected within the detectable region 301 are most likely to be captured by the detection system 40 of the imaging system 10.
  • the observation depth, denoted as 308, is the distance from the surface of an object, denoted as 307, to the focal plane of the imaging system 304.
  • Figure 3A and 3B show a schematic view of how the illumination beam 310 overlaps with the detectable region 301 in prior art microscopes, specifically, A) in the Oblique Illumination; B) in the Dark Field Illumination. It is noted that the Dark Field Illumination is a special case of the Oblique Illumination where the directly reflected light are not detected by the microscope.
  • this disclosure is to avoid or reduce the undesired light-tissue interactions that generate noise, particularly in the detectable region 301.
  • FIG 4 shows a schematic view of the Off-COL Side Illumination, which is an embodiment of the present invention.
  • the Off-COL Side Illumination carefully controls illumination beam path 310 to be outside of the detectable region or COL 301, either completely or as much as possible except nearing the target region around the FOV 302.
  • the illumination system 30 is arranged to project a projected beam spot 320 substantially displaced from the center of the FOV 302.
  • the displacements can be perpendicular to and/or along the axis 306 of the imaging system, which is respectively denoted as 321 and 323.
  • the plane parallel to the focal plane 304 that contains the focal point of the illumination beam is denoted as 322.
  • the Off-COL Side Illumination still directly illuminates a large amount of unrelated regions outside the detectable region or COL 301 on its way towards the target region 302.
  • the noise-forming light redirected from the outside of the detectable region or COL is less likely to be detected by the imaging system such as a microscope than that from the inside.
  • the Off-COL Side Illumination design compared with the prior art system shown in Figures 3A and 3B, can substantially reduce the direct illumination of the unrelated region inside the detectable region or COL (the shaded region), especially with the increased displacements 321, either perpendicular to and/or along the axis 306 of the imaging systems, between the center of the projected beam spot 320 and the center of the FOV 302.
  • the portion of the detectable region that is under direct illumination may be less than 25% of the total detectable region of the imaging system.
  • the Off-COL Side Illumination can reduce the undesired light-tissue interactions that otherwise could contribute substantial background noises. It can improve the image sharpness and the signal-to-noise ratio by preventing a large amount of the background noises from generation.
  • Figure 5 shows a schematic view of the Pinpoint Illumination, in which an illumination system design is used to focus the illumination beam 310 such that the projected beam spot 320, when projected onto the focal plane of the imaging system such as objective lens 304, is substantially smaller in size than that of the FOV 302.
  • the projected size of the illumination beam spot 320 at the target region may be less than a quarter size of the FOV 302 of the imaging system.
  • the Pinpoint Illumination can illuminate from the side (shown in Figure 5) or from the top (not shown).
  • the Pinpoint Illumination compared with the prior art shown in Figures 3A and 3B, substantially reduces the direct illumination of unrelated regions both inside and outside of the detectable region by using a much narrower illumination beam. It substantially reduces a large amount the undesired light-tissue interactions that otherwise could contribute substantial the background noises in the resulted images.
  • the Pinpoint Illumination and the Off-COL Side Illumination can be combined to achieve the benefits of both. This system and method is called the Pinpoint Off-COL Side Illumination, an example of which is shown on Figure 5.
  • Figure 6 discloses a beam controller system 326 according to the principles of the present invention, to allow user to control the aiming and other parameters of the above mentioned illumination systems.
  • the aiming parameters of illumination beam 310 that can be controlled includes: 1) the oblique angle 324 of the axis 325 of the illumination beam 310, relative to the axis 306 of the imaging system such as objective lens; 2) the (center) displacements 321 and 323, of the projected beam spot 320 relative to the FOV 302 ; 3) the size of the projected beam spot relative to the FOV.
  • the other parameters that can be controlled include wavelength, intensity, phase, and/or polarization of the illumination beam (not shown in Figure 6). All of these parameters can be fixed in the design of the disclosed illumination systems. However, making some parameters user adjustable through the beam controller 326 allows users to achieve optimal imaging result (e.g., in term of image sharpness, or, signal-to-noise ratio) on a case by case basis, and to aim at different regions of interest.
  • the Off-COL Side Illumination disclosed above differs from the Oblique Illuminations used in Dark-Field Microscope in following aspects: Oblique Illumination only refers to the case in which the illumination beam 310 and the axis 306 of the imaging system are not parallel. Dark-Field Microscope only refers to the case in which the illumination beam 310 and the axis 306 of the imaging system has a large enough angle to prevent the light directly reflected near the surface layers of the object 307 from being detected. Prior art methods say nothing about reducing the direct illumination within the detectable region 301 of the imaging system. Furthermore, prior art does not distinguish the region of FOV 320 from the region of the projected beam spot 320 and typically designs these two regions to be fixed and co-centered.
  • the Off-COL Side Illumination is designed to reduce the redirected light (including reflected as well as scattered, and other) from being generated in the unrelated region inside the detectable region 301, which includes both the surface layers 307 and underneath.
  • One way to achieve this reduction is to design a system to distinguish the region of FOV 302 from the region of the projected beam spot 320.
  • the projected beam spot 320 is designed to operate primarily off the center of the FOV 302, by either a fixed design or a user adjustable design ( Figure 6).
  • an aspect of this invention considers reducing the background noises as a higher priority requirement than maintaining illumination uniformity. It is noted that as the illumination light travels deeper and deeper into the tissue, it is more and more likely to be redirected by light-tissue interactions, more and more diffused from its projected (i.e. original) beam path. Thus, the selective (i.e., non-uniform) illumination featured by the off-center and/or Pinpoint Illumination works more effectively and selectively on the unrelated regions near the tissue surface 307 than towards the target region 309 deep into the tissue. As a result, the off-center and/or Pinpoint Illumination reduces the background noises generation more effectively and more selectively, and reduces the signal generation less effectively and less selectively. Thus, the off-center and/or Pinpoint Illumination substantially improves the overall image sharpness and the signal-to-noise ratio.
  • the intensity uniformity of the images from the off-center and/or Pinpoint Illumination may be compromised.
  • this compromise can be alleviated by providing the user controllable beam aiming ( Figure 6) so that user can aim at different regions of interest.
  • the different regions in the FOV depending on how far off the axis of the illumination beam 325, represents different tradeoffs of signal intensity and the signal-to-noise ratio,.
  • users can adjust this tradeoff interactively to get desired results.
  • users can obtain different images by adjusting the direction of the illumination beam 325, each optimized for different considerations (e.g., signal intensity or the signal-to-noise ratio) respectively.
  • Figure 7 discloses an embodiment of optics design that implements several embodiments of the present invention shown in Figures 4-6.
  • the illumination optics 30 includes: l)a light source 335 comprising an illuminant source 334 and a light condenser 333; 2) the beam controller 326 including a focusing adjustment 332, a illuminating aperture diaphragm 331, a light path controller 330, and the outer region of the objective lens 351.
  • the oblique angle 324 of the illumination beam can be adjusted by the light path controller 330.
  • the projected beam spot 320 can be adjusted by the light path controller 330 that controls the displacement 321 perpendicular to the axis of the imaging system 306, and/or by the focusing adjustment 332 that controls the displacement 323 along the axis of the imaging system 306.
  • the size of the projected beam spot 320 can be adjusted by the illuminating aperture diaphragm 331 and/or the focusing adjustment 332.
  • the detection optics 40 include: 1) the objective lens 351, with the FOV 302 defined by it; 2) a tube lens 328; 3) optionally, an imaging aperture diaphragm 327.
  • the objective lens 351 and the tube lens 328 combined defines the image plane 329.
  • the system 10 can be on tabletop or portable. It includes one or multiple Illumination Systems 30.
  • An Illumination Systems 30 includes, but is not limited to, one or multiple illuminant sources 334, one or multiple light condensers 333, one or multiple beam controllers 326 (controlling beam aiming and other properties), and a group of lens and various filters.
  • Multiple illumination beams 310 can illuminate at the objects at the same or different times, using the same or different imaging methods 20, with the same or different illumination methods, with the same or different beam parameters (e.g. beam angle, position, intensity, etc).
  • two illumination beams 310 can illuminate two targets (objects), respectively, one pinpointed to a specific target (a selected region in the FOV 302), and the other providing a more uniform illumination over the entire FOV.
  • the illuminant source 334 of this system can use all kinds of light or wave source with any types and principles. It includes, but is not limited to, halogen lamp, mercury lamp, xenon lamp, light emitting diode, and laser diode/ laser device etc.
  • the light may be polarized or unpolarized.
  • the light may have one or more specific wavelengths or wavelength ranges. It includes, but is not limited to, visible light, ultraviolet, or infrared light, ultrasound wave.
  • the illumination source 334 or 335 may be attached to a positioning device to ensure the correct position of light source.
  • This device may include a platform that can be adjusted and translated in all directions to correctly position the light source.
  • the positioning device may be controlled internally and/or by users.
  • the light condenser 333 includes, but is not limited to, one or more lenses, one or more adjustable diaphragms and various additional filters. Furthermore the Graded-Index or Gradient Index (GRIN) lens and light guide can be utilized in the light condenser 333.
  • the purpose of the light condenser 333 is to direct the light emitted by the illuminant source 334 to the next module such as the beam controller 326.
  • a focusing mechanism may be designed for the light condenser 333 to adjust the focal length of the illumination system.
  • the beam controller 326 may include, but is not limited to, one or more focusing adjustment lens 332 to adjust the focal length of the illumination system; one or more illuminating aperture diaphragm 331 to adjust the illumination beam width; and one or more light path controller 330 to change the beam direction.
  • the light path controller 330 may include a group of prisms or flat (inclined) mirrors.
  • the purpose of the beam controller 326 is to direct the illumination beam onto the selected region of the target region with desired illumination parameters.
  • the beam controller 326 may have one or more controlling devices to allow one or more beam parameters (such as aiming and focusing parameters) to be controlled internally and /or by users.
  • the objective lens system 351 is a part of the detection systems 40 that captures the redirected light rays from the target object.
  • the objective lens system should include, but is not limited to, a group of lenses and one or more diaphragms.
  • the objective lens system can be designed to have a selected magnification, a selected imaging aperture and a selected working distance.
  • the objective lens system may also be used as a part of the illumination systems 30 (e.g., a part of the beam controller 326 or the light condenser 333) to focus the illumination beam, one embodiment of which is shown in Figure 7.
  • the focusing used by the illumination beam may be either a separate lens (system) inside the same housing of the objective lens or (as shown in Figure 7) the separate region on the same objective lens.
  • the illumination region can use either the side region (as shown in Figure 7) or the center region of the objective lens, while the detection region using the other region.
  • the embodiment of providing illumination from inside the housing of the detection optical device such as objective lenses is called the internal illumination embodiment.
  • this disclosure can be implemented with a so-called external light illumination embodiment, where the illumination light is directed by a light guide external to (i.e., outside of) the objective lens of the microscope.
  • external light guide include, but are not limited to, fiber optics, LED diode, or separate lens system.
  • the objective lens system may be attached with an additional anaberration system. Aberration is produced when the target is covered by extra superstratum.
  • the anaberration system may be designed as an adjustable device, with one of the objective lens system being moved along the axial direction, in order to adapt to different situations.
  • the anaberration system may also be designed as a fixed device, for example, by taking extra superstratum into account when designing the objective lens.
  • the objective lens may be designed as an achromatic objective, an apochromatic objective, a semi-apochromatic objective, or a plan objective etc.
  • the objective lens can be designed as infinity conjugated or of a limited conjugated distance.
  • the objective lens may be designed as an immersion system.
  • the immersion medium may be oil, water, etc.
  • One exemplary use for the invention is the application in high-resolution human skin capillary microscopy observation.
  • the method is adopted to reduce the background noises in the resulted images.
  • the illumination light is compressed into a parallel beam that has a diameter which is much smaller than the clear aperture of an objective lens.
  • the illumination condenser system 333 includes an aperture diaphragm and a field diaphragm which are both adjustable. The luminous flux and the beam diameter can then be controlled according to the needs of the experiment.
  • the light condenser system 333 guides the illumination beam to enter the beam controller 326.
  • the beam controller 326 includes a group of optical catopters and stray light elimination diaphragms.
  • the beam controller 326 also includes a set of precision mechanical devices. Some of the catopters can be moved and rotated by such mechanical devices. Thus, the position and angle of the illumination beam can be controlled.
  • An infinite conjugate distance microscope objective lens unit 351 has a design with a numerical aperture value of 0.95 and a magnification value of 20x.
  • This objective lens unit 351 includes a diaphragm which is used to separate the regions between the illumination and the detection.
  • the illumination beam is directed by the beam controller 326 to enter the objective lens at the illumination region of the clear aperture.
  • the incident axis is tilted in relation to the centre axis of the objective lens. The angle of the incident axis is adjusted by the beam controller 326 .
  • the illumination beam can be converged by the objective lens to project onto the region near the FOV as a small spot. Adjusting the projected beam spot 320 by controlling the beam controller 326 will cause a selected target region to be illuminated. The lighting effects can be different if the projected beam spot is in a different position relative to the target.
  • the objective lens unit 351 has an imaging anaberration design. A method to correct this takes into account the refractive index and the thickness of the additional covering layer into an imaging formula.
  • Images can be observed by suitable eyepieces and they can also be recorded by a digital camera system.
  • a software analysis may be applied to measure the velocity of flow inside blood vessels and to estimate the diameter of a capillary.

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EP10843550A 2009-12-22 2010-12-21 Beleuchtungsverfahren und systeme zur verbesserung der bildauflösung von bildgebungssystemen Withdrawn EP2517064A2 (de)

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US95909410A 2010-12-02 2010-12-02
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