WO2008050254A1 - A system for imaging an object - Google Patents
A system for imaging an object Download PDFInfo
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- WO2008050254A1 WO2008050254A1 PCT/IB2007/054181 IB2007054181W WO2008050254A1 WO 2008050254 A1 WO2008050254 A1 WO 2008050254A1 IB 2007054181 W IB2007054181 W IB 2007054181W WO 2008050254 A1 WO2008050254 A1 WO 2008050254A1
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- Prior art keywords
- objective lens
- electromagnetic radiation
- lens
- image
- objective
- Prior art date
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- 238000003384 imaging method Methods 0.000 title claims abstract description 45
- 230000005670 electromagnetic radiation Effects 0.000 claims abstract description 62
- 230000003287 optical effect Effects 0.000 claims description 37
- 238000000034 method Methods 0.000 claims description 29
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Classifications
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- G—PHYSICS
- G02—OPTICS
- G02B—OPTICAL ELEMENTS, SYSTEMS OR APPARATUS
- G02B21/00—Microscopes
- G02B21/0004—Microscopes specially adapted for specific applications
- G02B21/002—Scanning microscopes
- G02B21/0024—Confocal scanning microscopes (CSOMs) or confocal "macroscopes"; Accessories which are not restricted to use with CSOMs, e.g. sample holders
- G02B21/0052—Optical details of the image generation
- G02B21/0076—Optical details of the image generation arrangements using fluorescence or luminescence
-
- G—PHYSICS
- G02—OPTICS
- G02B—OPTICAL ELEMENTS, SYSTEMS OR APPARATUS
- G02B21/00—Microscopes
- G02B21/0004—Microscopes specially adapted for specific applications
- G02B21/002—Scanning microscopes
- G02B21/0024—Confocal scanning microscopes (CSOMs) or confocal "macroscopes"; Accessories which are not restricted to use with CSOMs, e.g. sample holders
- G02B21/0032—Optical details of illumination, e.g. light-sources, pinholes, beam splitters, slits, fibers
Definitions
- the invention relates to a device for imaging an object.
- the invention further relates to an apparatus for imaging an object.
- the invention relates to a method of imaging an object.
- Optical imaging systems may be used in many different technical fields, for instance in the field of medical devices.
- US 2004/0223226 discloses a multiple-axis imaging system having individually-adjustable optical elements.
- the system comprises a plurality of optical elements having respective optical axes and being individually disposed with respect to one another to image respective sections of an object, and a plurality of individually-operable positioning devices corresponding to respective optical elements for positioning the optical elements with respect to their respective optical axes.
- the positioning devices are specifically adapted to adjust the axial position, lateral position and angular orientation of the optical elements with respect to their respective optical axes.
- the system is particularly adapted for use as a microscope array, and the positioning devices may be micro-actuators.
- a device for imaging an object comprising an objective lens adapted to manipulate a beam of electromagnetic radiation after interaction with, particularly transmitted through (alternatively reflected at), the object, a collimator lens adapted to manipulate the beam of electromagnetic radiation transmitted through the objective lens, and an actuator adapted for displacing the objective lens in a direction essentially parallel and in at least one direction (that is to say in one direction or in two directions which may be perpendicular to one another) essentially perpendicular to a propagation direction of the beam of electromagnetic radiation between the objective lens and the collimator lens, wherein the objective lens and the collimator lens are arranged so that the beam of electromagnetic radiation between the objective lens and the collimator lens is essentially parallel.
- an apparatus for imaging an object comprising an array formed by a plurality of devices having the above mentioned features.
- a method of imaging an object comprises manipulating, by an objective lens, a beam of electromagnetic radiation after interaction with, particularly transmitted through (alternatively reflected at), the object, manipulating, by a collimator lens, the beam of electromagnetic radiation transmitted through the objective lens, displacing the objective lens in a direction essentially parallel to a propagation direction of the beam of electromagnetic radiation between the objective lens and the collimator lens thereby adjusting a focus setting, acquiring an image, subsequently displacing the objective lens in a direction essentially perpendicular to a propagation direction of the beam of electromagnetic radiation between the objective lens and the collimator lens, maintaining or re-adjusting the focus setting, acquiring another image, repeating these steps so as to collect a multiplicity of images, processing the collection of images to form an overall image, and arranging the objective lens and the collimator lens so that the beam of electromagnetic radiation between the objective lens and the collimator lens is essentially parallel.
- a computer-readable medium in which a computer program of imaging an object is stored which, when being executed by a processor, is adapted to control or carry out a method having the above mentioned features.
- a program element of imaging an object is provided, which program element, when being executed by a processor, is adapted to control or carry out a method having the above mentioned features.
- the term "program element" may particularly denote any software component which is capable of controlling the scanning, signal detection and/or signal processing scheme for imaging an object under investigation.
- Signal processing and component control for improving image quality and/or operation speed which may be performed according to embodiments of the invention can be realized by a computer program, that is by software, or by using one or more special electronic optimization circuits, that is in hardware, or in hybrid form, that is by means of software components and hardware components.
- a microscope having an objective lens and a collimator lens, the objective lens being actuable in a direction parallel to a beam path and in one or both directions perpendicular thereto, so that an object to be imaged (for instance a tissue sample) may be scanned even with a single objective lens and a single actuator.
- an object to be imaged for instance a tissue sample
- a single objective lens and a single actuator By designing the optical system in a manner that the beam of electromagnetic radiation between the objective lens and the collimator lens is essentially parallel, a detector and also the collimator lens do not have to be moved, so that only few elements and consequently only a low weight have has to be moved, allowing a faster, simpler and more accurate motion.
- the objective lens and the collimator lens may be arranged so that sub-beams of the beam of electromagnetic radiation originating from the same portion of the object and being directed towards the same portion of a detector are essentially parallel at least between the objective lens and the collimator lens.
- the design of the optical arrangement may be such that all beams related to one object point and focused to one image point on the detector are parallel between the objective lens and the collimator lens.
- Acquiring the multiplicity of images can be done by placing the object or the entire imaging system on a translation table, so that the object and imaging system can be displaced with respect to each other in the two directions perpendicular to the optical axis.
- An issue with such a method is that the movables parts are bulky, and according to an exemplary embodiment of the invention only a part of the imaging system is displaced, namely the objective lens. This allows greater speed of displacement.
- a technical measure which allows such a system to work is that the beam directly downstream of the objective lens is essentially parallel.
- the actuator for displacing the objective lens in the direction perpendicular to the propagation direction of the beam may be adapted for displacing the objective lens for scanning and imaging a corresponding portion of the object.
- a part of the image is imaged, and the image parts may then be put together for forming an entire image.
- a microscope array formed by a plurality of such microscopes may be provided. Then, each of the microscopes can scan an assigned portion of an object. It is also possible that a plurality of objects are scanned simultaneously.
- an object imaging device particularly a microscope
- a scanning system which is similar to optical storage (e.g. DVD) readout systems (see for instance J. Schleipen, B.H.W. Hendriks, S. Stallinga, "Optical Heads", Chapter “Encyclopedia of Optical Engineering”, pp. 1667 to 1693, Marcel Dekker, New York, 2003).
- optical storage e.g. DVD
- An exemplary field of application of exemplary embodiments of the invention is DNA cytometry.
- a microscope or a microscope array according to embodiments of the invention in DNA cytometry, it is possible to acquire an image in a fast manner, and with a high throughput (that is to say with a high value of scanned area per time unit).
- the mass to be moved by a motion mechanism for scanning an object may be kept small, since the parallel beam paths between objective lens and the collimator lens makes it possible to move only a small portion of the device, whereas the main mass may be kept fixed.
- the largest part of the optical imaging system may be kept spatially fixed, distortions along the optical path may be prevented.
- an array of microscopes is provided
- Actuators may move objective lenses of each of the microscopes in order to scan a corresponding portion of an object.
- the used actuators may be magnet coil systems. Activating the coil by a current or voltage signal may generate an electromagnetic force between the magnet and the coil which may, by force transmission (for instance using tiny wires), move the objective lenses as well.
- piezoelectric actuators or other kinds of actuators are possible as well.
- individual objective lenses that is exactly one objective lens per microscope.
- an array microscope for DNA cytometry for visualization of DNA in the (cell) nuclei for detection of cancer or other diseases.
- an array microscope may be provided in which each microscope comprises at least two lens elements (namely an objective lens and a collimator lens).
- Systems for displacing the at least one objective lens along the focus direction (that is to say along a propagation direction of the electromagnetic beam) and along at least one of the remaining directions orthogonal to the focus direction may be provided.
- such an array microscope may be used in DNA cytometry.
- a telescope-like optical configuration may be provided in which the beam between the objective lens and the collimator lens in front of a detector (for instance a CCD, charge coupled device) is substantially parallel.
- a detector for instance a CCD, charge coupled device
- This may allow for an image acquisition mode in which the objective lens is displaced in the direction orthogonal to the optical axis. If the intermediate beam is not substantially parallel, the image might shift over the detector.
- this principle may be applied to an array microscope (comprising a plurality of microscopes) but also to a single microscope in which the lateral displacement of the objective lens may be used to broaden the field by taking multiple images and stitching them together.
- a microscope may be provided comprising at least two lens elements (namely an objective lens and a collimator lens), containing means for displacing at least the objective lens in the focus direction and in at least one of the two directions orthogonal to the focus direction, wherein the beam in between the at least two lens elements may be substantially parallel.
- an array of microscopes may be provided wherein each microscope is designed in such a manner.
- a method of acquiring an image of a field larger than the field of the microscope may be provided by taking multiple images, each image being laterally displaced with respect to the others by displacing the displaceable lens element according to the above-described microscope (array) in the lateral direction, and subsequently stitching the multiple images together to form an overall image.
- This method can be applied particularly advantageously in DNA cytometry.
- cancer may be diagnosed histologically on tissue sections from biopsies obtained from macroscopically suspicious surfaces.
- the technique of DNA- cytometry is based on the presence of numerical and/or structural aberrations in the chromosomes in the nucleus of the cell (aneuploidy). These aberrations are only found in tumor tissue. Detection of DNA-aneuploidy allows for very early diagnosis of cancer, often years ahead of the histological diagnoses on biopsies. The stage of aneuploidy (or the amount of "excess" DNA material) is a measure for how far the cancer has developed.
- a brush or a fine needle biopsy may be taken and subsequently colored with Fuelgen-staining.
- This staining binds to the DNA of cells and allows for the determination of the amount of DNA present in the cell nucleus. This may be done via a measurement of the integrated optical density (IOD). From a histogram of IODs of all cells in the sample, the (possible existing) cancerous cells can be determined. Either a pre-selection of suspicious cells are measured (so called first protocol) or, alternatively, all cells in the sample are measured (so called second protocol).
- the first protocol needs a trained pathologist to do the pre-selection (labor- intensive) and is therefore expensive.
- all cells are measured and only the most suspicious cells are viewed by a pathologist.
- the IOD and an image of the cell is measured and stored. This makes the method much less labor intensive but as all cells have to be measured at several heights in the sample in order to obtain the right focused imaged of the cell, the technique is rather time consuming. Since for each slide the full microscope system and software is needed, this low throughput of slides makes the measurement expensive again.
- exemplary embodiments of the invention provide a system capable to measure the IOD of the nuclei of all cells in the sample at a high speed and image the cells and their nuclei at the same time in order to allow final visual inspection of the suspicious cells for control. More particularly, the sample may be imaged with an array of compact, cheap and simple microscopes.
- Exemplary fields of application of embodiments of the invention are cancer screening and early cancer detection based on fast in vitro DNA cytometry.
- the device may comprise one or more further objective lenses, wherein the objective lens and the further objective lens(es) may be grouped to form a pair/group of objective lenses.
- Such grouped objective lenses may be moved cooperatively so as to increase the efficiency of the system, and keep the effort for the moving mechanism as small as possible. Furthermore, by grouping such lenses, a plurality of lenses may be used simultaneously for transmitting electromagnetic radiation. This keeps measurement times short.
- the pair of objective lenses may be arranged to be displaceable in common by the respective actuators. In other words, only a single motion mechanism and a simple motion control may be sufficient, thereby reducing the efforts and size when designing the device.
- the device may comprise a phase plate arranged, in an electromagnetic radiation propagation direction, downstream of the objective lens.
- a phase plate may be arranged between the objective lens and the collimator lens.
- Such a phase plate may be placed in the back focal plane of the objective lens when the microscope is used for phase contrast applications.
- a wavelength filter particularly a high-pass wavelength filter, may be arranged in an electromagnetic radiation propagation direction, downstream of the objective lens. Such a wavelength filter may be arranged between the objective lens and the collimator lens. Such a (high-pass) wavelength filter may be implemented when the microscope is used for fluorescence contrast applications.
- the device may be adapted as a microscope.
- a microscope may be denoted as an imaging device which generates a magnified image of an object.
- the objective lenses of the devices may be staggered with respect to one another. More particularly, the pairs of objective lenses of the devices may be staggered with respect to one another. In other words, adjacent objective lens pairs (with individual lenses having a distance of 12 mm from one another) may be displaced by a specific distance, for instance by 1 mm. Therefore, it is possible to use the plurality of staggered objective lenses/lens pairs/lens groups to scan portions of the object, thereby making the analysis more efficiently and allowing for a high throughput analysis.
- the pairs/groups of objective lenses of the devices may be staggered with respect to one another along the direction essentially perpendicular to the propagation direction of the beam of electromagnetic radiation along which direction the pairs of the objective lenses of the devices are displaceable by the actuators. Therefore, the staggering direction and the lateral motion direction of the collimator lenses may be identical.
- the staggering distance may then be selected so that lateral oscillation of adjacent staggered lenses (or groups of lenses) allow to scan the object without invisible portions. A slight overlap of the scanned portions is possible and may simplify stitching together the individual image portions.
- the apparatus may comprise a motion mechanism adapted for displacing the objective lenses of the plurality of devices relative to the object in a direction essentially perpendicular to the direction essentially parallel and to the direction essentially perpendicular to the propagation direction of the beam of electromagnetic radiation.
- a motion mechanism for instance a linear stepper motor, may move the object (which may be mounted on a sample holder) and may keep the objective lenses spatially fixed. This may be advantageous, since a motion of the relatively heavy objective lenses may be avoided and these optical elements can be kept fixed.
- the objective lenses are moved and that the object (mounted on a sample holder) remains fixed. By moving objects or objective lenses perpendicular to the lateral displacement, a simultaneous scan of a plurality of objects is possible. Therefore, batches of objects may be investigated.
- the apparatus may comprise a sample holder adapted for holding one or a plurality of objects to be imaged. This may allow to perform a high throughput analysis.
- the motion mechanism may be adapted for displacing the sample holder to image the plurality of objects using the plurality of devices.
- the motion mechanism may displace the objective lenses of the plurality of devices relative to the object using a linear displacement or a relative rotation.
- a relative rotation (see Fig. 3) may be preferred since this may allow to avoid or reduce dead time.
- the various samples may be mounted on a rotatable wheel, and the lenses may be spatially fixed.
- the samples or objects may be spatially fixed, and the objective lenses may be mounted on a rotatable wheel.
- the apparatus may comprise an electromagnetic radiation source adapted to generate the beam of electromagnetic radiation to be directed to the object.
- Such an electromagnetic radiation source may be any kind of lamp, or a laser, etc.
- the electromagnetic radiation source may particularly be adapted to generate an essentially monochromatic beam of electromagnetic radiation.
- the term "essentially monochromatic” may denote that ⁇ « ⁇ , wherein ⁇ is the (average) wavelength of the electromagnetic radiation source and ⁇ is the spectral bandwidth of the electromagnetic radiation source.
- ⁇ is the (average) wavelength of the electromagnetic radiation source
- ⁇ is the spectral bandwidth of the electromagnetic radiation source.
- the electromagnetic radiation source may be adapted to generate an essentially parallel beam of electromagnetic radiation. It may be not or not only the illumination optics being a key to having parallel beams between objective and collimator. In fact, an exactly parallel illumination beam may be obtained for an ideal point source (for example a laser). In practice, a spatially extended source such as a LED or several types of lamps, may be used.
- the illumination then comes from (an infinitely large) number of point sources, each point source giving a parallel illumination beam at the object, the parallel beam making an angle with the optical axis proportional to the distance between the point source and the optical axis. Adding all parallel beams it then follows that an entire field of object points is illuminated, each object point in the field being illuminated by a converging cone of light, the top angle of the cone being determined by the illumination optics and the lateral extension of the light source.
- This type of illumination may be called K ⁇ hler- illumination and one type of illumination in microscopes (see M. Born and E. WoIf, "Principles of Optics", 6th edition, p. 522-526, Cambridge University Press, 1980, ISBN 0521639212).
- the electromagnetic radiation source may be adapted to generate the beam of electromagnetic radiation of at least one of the group consisting of optical light, infrared radiation, ultraviolet radiation, and X-rays.
- the optical light domain may include the wavelength region between 400 nm and 800 nm.
- the infrared radiation may include the wavelength region with wavelengths higher than those of optical light, and ultraviolet radiation has wavelengths shorter than those of optical light.
- X-rays may have energies in the order of magnitude of kilo electron volts (keV).
- keV kilo electron volts
- the use of optical light may be preferred for specific applications, like DNA cytometry.
- the apparatus may comprise a detector unit comprising an array of detector elements arranged to detect the beam of electromagnetic radiation transmitted through the collimator lens.
- a detector unit comprising an array of detector elements arranged to detect the beam of electromagnetic radiation transmitted through the collimator lens.
- Examples for such a detector unit is a CCD (charge coupled device) or a CMOS sensor array.
- the detector unit may be adapted to detect the image of the object and may be adapted to detect an integrated optical density (IOD).
- IOD integrated optical density
- the apparatus may be adapted to image the object for a plurality of focal positions. Taking this measure, for instance by allowing the object of lenses to be moved along the beam path, makes the apparatus appropriate for DNA cytometry applications.
- the device may be adapted to image tissue of a physiological object.
- physiological object may denote a human being, an animal or a plant. Therefore, biological information may be derived with the device, for example with in vivo or in vitro investigations.
- the device may be used in many different technical fields, for instance as a microscope, as a cytometry device (particularly as a DNA cytometry device), as a cancer detection device, as a cancer screening device, or as a high throughput screening device (for instance for biological, genetic or pharmaceutical applications).
- Other exemplary applications are a malaria screening device, a cell imaging device, array imaging, or a multi- well plate scanner.
- the method may further comprise adjusting a focus setting by displacing the objective lens in the direction essentially parallel to the propagation direction (between the objective lens and the collimator lens) of the beam of electromagnetic radiation, acquiring data related to an image of at least a portion of the object, subsequently displacing the objective lens in the direction essentially perpendicular to the propagation direction (between the objective lens and the collimator lens) of the beam of electromagnetic radiation, acquiring data related to another image of at least another portion of the object, and processing the data related to the image of the portion of the object and the data related to the other image of the other portion of the object to form an overall image of the object.
- multiple images of different portions of the object may be taken by moving the objective lens, and may then be stitched together to reconstruct a complete image of the object.
- the method may further comprise re-adjusting the focus setting (for instance by displacing the objective lens in the direction essentially parallel to the propagation direction) before acquiring the data related to the other image of the other portion of the object.
- re-adjusting the focus setting for instance by displacing the objective lens in the direction essentially parallel to the propagation direction
- Fig. 1 illustrates a device for imaging an object according to an exemplary embodiment of the invention.
- Fig. 2 illustrates an objective lens array of a device for imaging an object according to an exemplary embodiment of the invention.
- Fig. 3 illustrates an objective lens array of a device for imaging an object according to an exemplary embodiment of the invention.
- a microscope 100 according to an exemplary embodiment of the invention will be explained.
- the device 100 is adapted for imaging an object 101, namely a tissue sample.
- the device 100 comprises an objective lens 102 adapted to manipulate a beam of electromagnetic radiation 103 transmitted through the object 101. Further, a collimator lens 104 is provided to manipulate the beam of electromagnetic radiation 103 transmitted through the objective lens 102.
- An actuator 105 is provided for displacing the objective lens 102 in a direction essentially parallel and in at least one direction essentially perpendicular to a propagation direction of the beam of electromagnetic radiation 103 (according to Fig. 1, from left to the right) between the objective lens 102 and the collimator lens 104.
- the optical arrangement 100 and particularly the objective lens 102 and the collimator lens 104, are positioned and designed (regarding material, geometrical and optical properties) so that the beam of electromagnetic radiation 103 between the objective lens 102 and the collimator lens 104 is essentially parallel. More precisely, each object point 106a, 106b generates beam portions (see dotted lines and solid lines of the beam 103) which are manipulated by the optical elements 102, 104 in such a manner that corresponding image points 107a, 107b are focused on a detector 108. Particularly, the object point 106a is focused on the image point 107a. The object point 106b is focused on the image point 107b.
- a phase plate 109 may be optionally arranged, in the electromagnetic radiation propagation direction, downstream of the objective lens 102, particularly between the objective lens 102 and the collimator lens 104.
- the phase plate 109 may be substituted by a wavelength filter, particularly a high-pass wavelength filter, arranged, in an electromagnetic radiation propagation direction, downstream of the objective lens 102, particularly between the objective lens 102 and the collimator lens 104.
- Fig. 1 is a schematic view of an individual microscope element 100.
- Light is emitted by a light source 110. It is also possible that a plurality of light sources 110 are provided.
- the emitted beam of light 103 is made essentially parallel by a collimating lens 111, passes through a first substrate 112 of a sample holder and thereby illuminates the object layer 101.
- the light modified by the object layer 101 passes through a second substrate 113 of the sample holder, the objective lens 102 placed on the actuator 105, optionally the plate 109, the collimator lens 104, and is incident on the CCD detector 108, for instance a pixel detector such as a CCD.
- one or both of the substrates 112, 113 may be omitted.
- the sample 101 may be fixed at a single substrate or may be simply be placed in the beam path.
- the object plane 106a, 106b and the image plane 107a, 107b are optically conjugate, meaning that light 103 emanating from object point 106a is collected at image point 107a, and light 103 emanating from object point 106b is collected at image point 107b.
- the actuator 105 can adjust the focal position on the object 101 with respect to the microscope 100 and can displace the lens 102 in one of the directions perpendicular to the focus direction (which focus direction is a direction from the left-hand side of Fig. 1 to the right-hand side of Fig. 1).
- the plate 109 may be omitted when the microscope 100 is used for standard absorption contrast.
- the plate 109 may be a phase plate placed in the back focal plane of the objective lens 102 when the microscope 100 is used for phase contrast.
- the plate 109 may be a wavelength filter (high-pass) when the microscope 100 is used for fluorescence contrast.
- Fig. 1 shows the optical setup of an individual microscope element 100 including the objective lens 102 placed on the actuator 105 and the image sensor 108 (CCD or a CMOS sensor).
- the image sensor 108 CCD or a CMOS sensor
- the actuator 105 (which can move the lens 102 along the focus direction and along one of the directions perpendicular to the focus direction, for example perpendicular to the paper plane of Fig. 1) can be an actuator as implemented in the field of optical data storage.
- the image sensor 108 can have a relatively low resolution (for instance 0.25
- the sample 101 may be illuminated with a broad parallel monochromatic beam 103.
- the objective lens 102 may be used for red light (655 nm), but it can also function with sufficient quality at a difficult wavelength, like green light (about 500 to 600 nm). However, since the objective lens 102 cannot work simultaneously for these wavelengths with the highest accuracy, it may be advantageous that the illumination is essentially monochromatic.
- a throughput of an array microscope 100 for instance the one shown in Fig. 2 can be estimated as follows:
- Fig. 2 shows a plan view of a part of an apparatus 200 for imaging the object 101.
- the apparatus 200 comprises a plurality of devices 100 according to the above- described Fig. 1.
- Fig. 2 shows a coordinate system with axes x, y and z, wherein x is a direction along which the collimator lenses 102 are displaceable.
- the y-direction indicates a direction along which, as will be described below in more detail, samples 105 may be shifted, for instance using a stepper motor.
- the direction z corresponds to the horizontal direction of Fig. 1, that is to say the general propagation direction of the beam 103. In other words, the beam 103 propagates out of the paper plane of Fig. 2. Above the paper plane of Fig. 2, the detector 108 is positioned.
- Fig. 2 shows a plurality of samples 101. All of these samples may be scanned in a common procedure.
- the circle around reference numerals 102 denotes a lens
- the surrounding rectangle 201 denotes a lens mount.
- Springs (tiny wires) 202 connect the lenses 102 with actuator magnets 203.
- the magnets 203 cooperate with coils (not shown) to generate electromagnetic forces which may have an impact on the springs 202 to move the lens 102 in the x-direction and/or in the z-direction.
- two collimator lenses 102 are grouped to form a group of a pair of objective lenses 102, 102.
- the respective groups of objective lenses 102, 102 are displaceable in common/in a correlated manner by the actuator 203.
- a first sample 211 passes a first pair of lenses 102, 102.
- a third sample 231 passes a third microscope unit 230 comprising a third pair of lenses 102, 102. This pair 102, 102 is staggered by about 1 mm with respect to the second pair of lenses 102, 102, and so on.
- a twelfth sample 241 passes a twelfth microscope unit 240 comprising a twelfth pair of lenses 102, 102 shown at a bottom part of Fig. 2. These lenses 102, 102 finalize the system, so that the whole area of the sample 101 has been imaged.
- Fig. 2 shows an example of an array microscope 200 using 24 actuators 203 and using 24 objective lenses 102.
- the objective lenses 102 are placed in twelve pairs.
- About 14 to 15 images of 70 ⁇ m x 70 ⁇ m can thus be taken by laterally displacing the lens 102.
- the second pair of lenses 102, 102 is staggered with respect to the first pair 102, 102 by about 1 mm, the third pair 102, 102 by about 2 mm, etc., until the twelfth pair 102, 102.
- Fig. 3 shows an array microscope 300 using 24 actuators 203. It is possible to rotate the samples 101 and to keep the optical arrangement 100 fixed. Alternatively, it is possible to rotate the optical arrangements 100 and to keep the samples 101 fixed.
- a method of using the microscope arrays 200, 300 for DNA cytometry will be explained. The following steps may be carries out.
- the microscope functions with a different contrast mechanism (see Fig. 1). For example, placing a high-pass wavelength filter in the light path, the microscope can be easily adapted for a fluorescence contrast. Similarly, by placing a phase plate in the light path the microscope can be easily adapted for phase contrast. Images of the sample can be made with an absorption contrast method, with fluorescence contrast and/or with phase contrast in order to improve the accuracy of the image analysis processed that determines the IODs for the nuclei of the cells.
- the imaging system is operated in a transmission mode.
- an imaging system according to an exemplary embodiment may be operated in a reflection mode or in a fluorescence mode (for instance using epi illumination).
Abstract
Description
Claims
Priority Applications (4)
Application Number | Priority Date | Filing Date | Title |
---|---|---|---|
EP07826738A EP2076809A1 (en) | 2006-10-24 | 2007-10-15 | A system for imaging an object |
JP2009533994A JP2010507828A (en) | 2006-10-24 | 2007-10-15 | System for imaging an object |
BRPI0717385-7A BRPI0717385A2 (en) | 2006-10-24 | 2007-10-15 | DEVICE, APPARATUS AND METHOD FOR FORMING PICTURE OF AN OBJECT |
US12/446,462 US20110001036A1 (en) | 2006-10-24 | 2007-10-15 | system for imaging an object |
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EP06122861 | 2006-10-24 | ||
EP06122861.5 | 2006-10-24 |
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US (1) | US20110001036A1 (en) |
EP (1) | EP2076809A1 (en) |
JP (1) | JP2010507828A (en) |
CN (1) | CN101529304A (en) |
BR (1) | BRPI0717385A2 (en) |
RU (1) | RU2009119425A (en) |
WO (1) | WO2008050254A1 (en) |
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Also Published As
Publication number | Publication date |
---|---|
RU2009119425A (en) | 2010-11-27 |
US20110001036A1 (en) | 2011-01-06 |
CN101529304A (en) | 2009-09-09 |
JP2010507828A (en) | 2010-03-11 |
BRPI0717385A2 (en) | 2013-10-15 |
EP2076809A1 (en) | 2009-07-08 |
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