AU2002303160B2 - Apparatus and method for imaging small objects in a flow stream using optical tomography - Google Patents
Apparatus and method for imaging small objects in a flow stream using optical tomographyInfo
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Description
APPARATUS AND METHOD FOR IMAGING SMALL OBJECTS IN A FLOW STREAM USING OPTICAL TOMOGRAPHY
Related Application
This application is related to co-pending provisional application of Alan C. Nelson, serial number 60/279244, filed 03/28/2001, entitled "APPARATUS AND METHOD FOR IMAGING SMALL OBJECTS IN A FLOW STREAM USING OPTICAL TOMOGRAPHY," and, by this reference, claims the benefit of the priority filing date of the co-pending provisional application. Background ofthe Invention The present invention relates to three dimensional optical tomography using point source projection geometry, and, more particularly, to imaging microscopic objects, including biological cells, in a flow stream using optical tomography.
With the advent of molecular probes, such as antibody probes and nucleic acid hybridization probes, new disease related questions can be addressed by tagging these molecular probes and then measuring their location and concentration within biological cells and tissues. As the need to more accurately localize and quantify these probes is emerging, there is a concomitant need for improved techniques to measure probe densities microscopically in two dimensions (2D) and three dimensions (3D). Traditional light microscopy, which utilizes cells mounted on glass slides, can only approximate 2D and 3D because of limitations in focal plane depth, sampling angles, and problems with cell preparations that typically cause cells to overlap in the plane of the image. Another drawback of light microscopy is the inherent limitation of viewing through an objective lens where only the area within the focal plane provides accurate data for analysis.
Flow cytometry methods generally overcome the cell overlap problem by causing cells to flow one-by-one in a fluid stream. Unfortunately, flow cytometry systems do not generate images of cells of the same quality as traditional light microscopy, and, in any case, the images are not three dimensional. For background, those skilled in the art are directed to Shapiro, HM, Practical How Cytometry. 3rd ed., Wiley-Liss, 1995.
In the area of computer aided tomography, US Patent No. 5,402,460, issued March 28, 1995, to Johnson, et al. entitled "Three dimensional Microtomographic Analysis System" discloses a microtomographic system for generating high-resolution, three dimensional images of a specimen using an x-ray generator and an x-ray detector that measures the attenuation of the x-ray beam through the specimen. Two projections, each using a different energy x-ray beam, of each view ofthe specimen are made with Johnson, et al.'s microtomographic system. After the two projections of one view of the specimen are made, the specimen is rotated on the specimen holder and another set of projections is made. The projections of each view of the specimen are analyzed together to provide a quantitative indication ofthe phase fraction ofthe material comprising the specimen. The projections of the different views are combined to provide a three dimensional image of the specimen. US Patent No. 5,402,460 is incorporated herein by reference. Although the x-ray technology as taught by US Patent No. 5,402,460 is useful for some applications, it does not provide an optical solution useful for flow cytometry. To overcome the aforementioned limitations and others found in such systems, it is a motivation of this invention to combine the one-by-one cell presentation of flow cytometry with computational optical tomography from multiple point source projections to reconstruct 2D and 3D cell density information from a plurality of projections.
Summary ofthe Invention
The invention provides an apparatus and method for imaging small objects in a flow stream using optical point source projections and tomographic image reconstruction.
The flow optical tomography (FOT) system includes a flow cytometer, as shown in FIG. 1, and a reconstruction cylinder, as shown in FIG. 4, positioned around capillary mbe 2. A source of photons 25 and a photon sensor 26 work together with pulse height analyzer 27 to operate as a triggering device. Pulse height analyzer 27 operates in accordance with known principals to provide a first trigger point 28 for the beginning of a cell, and a second trigger point 29 for the end of the cell. The pulse height analyzer 27 outputs a trigger signal 30 corresponding to the beginning and end of each cell, where the trigger signal is received by the reconstruction cylinder 20. Signals from the reconstruction cylinder may be analyzed directly or processed using computerized tomographic image reconstruction techniques to provide two or three dimensional information about cells.
Brief Description ofthe Drawings FIG. 1 schematically shows an example illustration of a flow cytometry system as contemplated by an embodiment ofthe present invention.
FIG. 2 schematically shows an example illustration of a flow process for a single cell as contemplated by an embodiment ofthe present invention.
FIG. 3 A and FIG. 3B schematically show an example of a cell and a cross-section of reconstruction as contemplated by an embodiment of the present invention.
FIG. 4 schematically shows an example of a reconstruction cylinder as contemplated by an embodiment of the present invention.
FIG. 5 schematically shows an example of a flow optical tomography tJFOT) system as contemplated by an embodiment ofthe present invention.
FIG. 6 schematically shows an example of projection rays within a reconstruction cylinder as contemplated by an embodiment ofthe present invention. FIG. 7 schematically shows an example of a top view of a reconstruction cylinder as contemplated by an embodiment ofthe present invention.
FIG. 8 schematically shows an example of the geometry of a source/linear array configuration used in cell reconstruction as contemplated by an embodiment ofthe present invention. Detailed Description ofthe Preferred Embodiments
The invention is described herein with respect to specific examples relating to biological cells, however, it will be understood that these examples are for the purpose of illustrating the principals ofthe invention, and that the invention is not so limited. In one example, constructing a three dimensional distribution of point densities and emission intensities within a microscopic volume allows the measurement of density and fluorescence at any location within the microscopic volume and determines the location of structures, molecules or molecular probes of interest. By using tagged molecular probes, the quantity of probes that attach to specific structures in the microscopic object may be measured. For illustrative purposes, an object such as a biological cell may be labeled with at least one tagged molecular probe, and the measured amount and location of this probe may yield important information about the disease state of the cell, including, but not limited to, various cancers such as lung, breast, prostate, cervical and ovarian cancers.
Biological cells that have been prepared for flow cytometry and stained or labeled with tagged molecular probes for specific disease diagnosis, are caused to flow through a cylindrical device that provides for the projection image and allows the reconstruction of 2D and 3D density information from optical projection ray paths approximately peφendicular to the flow vector ofthe cell. By controlling the velocity ofthe cell flowing along an axis, the peφendicular 2D planes of reconstruction can be correctiy located (or stacked) along the axis ofthe cell to create a 3D picture ofthe entire cell, or a 3D image of the cell may be computed directly from 2D optical transmission or emission projections. Flow cytometry is highly suitable for image reconstruction because of the following characteristics:
• cells flow in single file through the capillary tube so cell overlapping and obscuration are minimized,
• the velocity of cells flowing through the capillary tube can be directly measured and is constant,
• cells tend to follow the center axis of the capillary tube and become structurally radially symmetric, and
• depending on the cell fixation and suspension preparation, cells can retain plasticity and assume an elongated shape along the z-axis in response to the velocity gradient in the capillary tube.
The present invention takes advantage ofthe aforesaid characteristics to provide a system for point source projection imaging and tomographic image reconstruction.
Referring now to FIG. 1, there shown schematically is an example illustration of a flow cytometry system as contemplated by an embodiment of the present invention. The system is oriented with reference to a coordinate system 11 having coordinates in the x, y and z-directions. In operation, cells 1 are injected into injection tube 3 using a known injection device 4. The capillary tube is wider at an injection end 5 and includes a pressure cap 6. A sheath fluid 7 is introduced at tube 8 to create laminar flow within the capillary tube 2. It is characteristic of traditional flow cytometry that the cells 1, prepared and suspended in solution, can be forced through a capillary tube 2 such that they elongate with the axis of flow and move approximately down the central axis of the capillary tube 2, as represented by dashed line 9. Cells may advantageously be made to flow with axial symmetry and with constant velocity 10 in single file along the center axis of a cylindrical capillary tube.
Referring now to FIG. 2, there shown schematically is an example illustration of a flow process for a single cell as contemplated by an embodiment ofthe present invention. A cell 1 moves with a constant velocity (V) indicated by velocity vector 10 through a capillary tube 2. The cell 1 comprises a wall of cell cytoplasm 12 and a wall of cell nucleus 13. During the course of flowing through the capillary tube 2, the cell 1 passes through a plurality of reconstruction planes represented for illustrative puφoses as first, second and third reconstruction planes 14a, 14b and 14c respectively. A first planar slice 15a through the wall ofthe cell cytoplasm lies within reconstruction plane 14a. Similarly, a second planar slice 15b through the walls ofthe cell cytoplasm and the cell nucleus, lies within the second reconstruction plane 14b, and a third planar slice 15c lies within the third reconstruction plane 14c. A central feature of the present invention is that a number
of optical point sources of selectable wavelength are disposed about and concentric with the capillary tube. The optical point sources operate in conjunction with opposing optical sensor arrays that are sensitive to selectable portions of the light spectrum, thus allowing the acquisition of projections of the light transmitted through the cell. The acquired projection images may be analyzed directly or processed using tomographic image reconstruction algorithms to provide spatial maps or images ofthe distribution of densities and/or emission intensities within the cell. It will be understood that in practice the number of reconstruction planes may vary from several to several hundred or more, depending on the needed image resolution ofthe object being presented to the system. The group of reconstructed parallel planar slice images may be combined or stacked in software to produce a three dimensional (3D) image of the densities and emission intensities within the cell. In addition, by employing planar (2D) instead of linear (ID) light sensor arrays, and a cone instead of a fan illumination ray pattern, projections of a plurality of contiguous planar slices through the flowing cells may be acquired simultaneously. As a result, three dimensional (3D) images ofthe distribution of densities and emission intensities within the cell volume can be computed directiy from the two dimensional (2D) projections using cone-beam reconstruction algorithms. Alternatively, the 2D point source projection images, which possess infinite depth of field, can be analyzed directly. In the case of a biological cell, a distance (d) between reconstruction planes may be a few microns or less. A point within the cell 1 will coincide with each reconstruction plane at time intervals, where the time intervals (t) may be described according to the relationship:
t = d ÷ N (Equation 1).
Referring now jointly to FIG. 3A and FIG. 3B, there shown schematically is an example of a cross-section 16 of reconstruction as contemplated by an embodiment ofthe present invention. Reconstruction of point densities within a cell from optical projections through it benefits from the axial symmetry and centrality of the flowing cell. Additionally, the space being sampled by projections can be modeled as consisting of three discrete compartments:
1. the fluid outside the cell 17 (i.e. the sheath fluid or cell suspension medium),
2. the cell cytoplasm 18, and 3. the cell nucleus 19.
Knowing quantitatively the distribution of optical density or molecular probes in these three compartments is sufficient to address many important problems in cell biology and disease diagnosis. Additionally, it may be useful to compute two boundary surfaces including the cytoplasmic or cell wall 12 and the nuclear wall 13 if certain molecular probes bind preferentially to those surfaces. Otherwise, it may be sufficient to characterize these walls as the transition surfaces between the three different compartments.
By combining the reconstructed slices ofthe cell, or by reconstructing in a helical, volumetric manner, the 3D moφhology and volume information can be generated, but absolute (as opposed to relative) volumes depend on accurate information of cell location. Cell location is a function ofthe flow velocity. However, in several instances, the relative concentrations of density or molecular probes are sufficient to address the diagnostic question: How much probe is in the cytoplasm relative to the nucleus vs. the non-bound
probe in the background fluid? Or, is the probe located primarily on the cell membrane or nuclear membrane surface?
While the cells passing through the capillary tube may become structurally radially symmetric, the distribution within the nuclear and cytoplasmic compartments of at least one bound molecular probe may not possess such axial symmetry. It is therefore desirable for the imaging system and (particularly the emission) reconstruction algorithm to provide sufficient spatial resolution to localize volumes of bound, fluorescing molecular probe on a scale finer than that required to provide the three compartment analysis described above. It is further desirable that the system provides quantitative information about the concentration of asymmetrically distributed probe within the two intracellular compartments. The association of the probe with specific subcellular compartments, structures or organelles within the cytoplasm or nucleus is facilitated by sub icron spatial resolution.
A more specific example pertains to the early detection of cancer in patients at risk. In such cases, certain genes may over or under express their function when the cell is undergoing transformation. It is diagnostically important to measure the relative over or under expression of the gene product (often a protein) in the cytoplasm relative to the nucleus, while normalizing for non-bound probes in the background suspension fluid. If the gene product is a protein, then a tagged antibody probe may be used to assess the disease state ofthe cell by localizing and/or quantifying the gene product protein. Hence, the three compartment analysis can be sufficient to make this the determination of disease state.
Referring now to FIG. 4, there shown schematically is an example of a reconstruction cylinder, surrounding flow tube 2 containing flowing cells 1, as contemplated by an embodiment of the present invention. A reconstruction cylinder 20 includes, for example, a helix 24 of point sources 21 disposed at a predetermined helical pitch, with pitch angle θ. Each point source 21 generates a beam of photons 22, where the beam of photons 22 is typically cone or fan shaped. While the arrangement ofthe sources depicted in the example of FIG. 4 is helical, the array of point sources may take on a wide variety of geometric patterns, depending in part on the speed of the electronics, the cell velocity and the geometry that achieves non-overlapping projection signals at the sensor (detector). Sensing elements 23 are disposed to receive light from the point sources.
The fixed optical point sources 21, in conjunction with opposing detectors 23 mounted around a circumference of the tube can sample multiple projection angles through the entire cell 1 as it flows past the sources. By timing ofthe emission or readout, or both, of the light source and attenuated transmitted and/or scattered and or emitted light, each detected signal will coincide with a specific, known position along the axis in the z-direction of the flowing cell. In this manner, a cell 1 flowing with known velocity along a known axis peφendicular to a light source that is caused to emit or be detected in a synchronized fashion, can be optically sectioned with projections through the cell that can be reconstructed to form a 2D slice in the x-y plane. By stacking or mathematically combining sequential slices, a 3D picture of the cell will emerge. It is also possible to combine the cell motion with the positioning of the light source (or sources) around the flow axis to generate data that can be reconstructed, for example, in a helical manner to create a 3D picture of the cell. Reconstruction can be done either by stacking contiguous
planar images reconstructed from linear (ID) projections using fan-beam reconstruction algorithms, or from planar (2D) projections directly using cone-beam reconstruction algorithms. The 3D picture of the cell can yield quantitative measures of sub-cellular structures and the location and amount of tagged molecular probes that provide diagnostic information.
As mentioned, more than one projection through a cell section is required to reconstruct the 2D or 3D density structure in the section or volume. In traditional slice-by- slice medical x-ray computed tomography, multiple projections are made by holding the human patient motionless while the x-ray source and opposing detectors move along a circumference to generate multiple projection angles through the patient. By analogy, the flow optical tomography system of this invention moves the cell at a predetermined velocity (V) past multiple sources positioned at different angles along the circumference of the capillary tube to generate multiple projections through the cell as it flows past the point sources. These point sources emit photons that pass through the cell and are detected by an array of sensors opposite the source. The point sources can be arranged along a helix 24, or in other appropriate geometric patterns, on the circumference of the capillary tube such that each point in the cell is sampled from a multitude of angles as it passes through the array of point sources. For good sampling geometry, these point sources may cover at least 180 degrees of circumference. Less angular coverage (i.e. angular under sampling) may be feasible in some instances, while additional radial coverage will improve accuracy and the signal-to-noise ratio ofthe computed reconstruction. Depending on the geometry, it may be advantageous to apply traditional analytical, iterative or statistical algorithms for cone-beam or fan-beam image reconstruction. (See, for example, Gilbert, P, "Iterative
Methods for the Three dimensional Reconstruction of an Object from Projections," Journal of Theoretical Biology 36:105-17, 1972, Oppenheim, BE, 'More Accurate Algorithms for Iterative 3 dimensional Reconstruction," IEEE Transactions on Nuclear Science NS-21:72-7, 1974, Singer, JR, Grunbaum, FA, Kohn, P, and Zubelli, JP, "Image Reconstruction of the Interior of Bodies that Diffuse Radiation," Science 248(4958) :990- 3, 1990. Mueller, K and Yage, R, "Rapid 3-D Cone-beam Reconstruction with the Simultaneous Algebraic Reconstruction Technique (SART) Using 2-D Texture Mapping Hardware", IEEE Transactions on Medical imaging 19(12):1227-37, 2001.) Related methods include, but are not limited to ART (algebraic reconstruction technique, as discussed in Bellman, SH, Bender, R, Gordon, R, and Rowe, JE, "ART is Science being A Defense of Algebraic Reconstruction Techniques for Three dimensional Electron Microscopy," Journal of Theoretical Biology 32:205-16, 1971), SIRT (simultaneous iterative reconstruction technique, as discussed, for example by Gilbert, id. #1493), ML- EM (maximum likelihood expectation maximization, as discussed, for example, by Manglos, SH, Jaszcak, RJ, and Floyd, CE, "Maximum Likelihood Reconstruction for Cone Beam SPECT: Development and Initial Tests," Physics in Medicine and Biology 34(12):1947-57,1989, #1382), and OSEM (ordered subsets expectation maximization, as discussed, for example, in Manglos, SH, Gagne, GM, Krol A, Thomas, FD, and Narayanaswamy, R, "Transmission Maximum-likelihood Reconstruction with Ordered Subsets for Cone Beam CT", Physics in Medicine and Biology 40(7):1225-41, 1995, #4389). METHODS: Flow Cytometer.
Referring now to FIG. 5, there shown schematically is an example of a flow optical tomography system (FOT) as contemplated by an embodiment of the present invention. The flow optical tomography system includes a flow cytometer, with a reconstruction cylinder 20 positioned around capillary tube 2. A source of photons 25 and a photon sensor 26 work together with pulse height analyzer 27 to operate as a triggering device. Pulse height analyzer 27 operates in accordance with known principals to provide a first trigger point 28 for the beginning of a cell, and a second trigger point 29 for the end ofthe cell. The pulse height analyzer 27 outputs a trigger signal 30 corresponding to the beginning and end of each cell, where the trigger signal is received by the reconstruction cylinder 20.
A computer 40 is coupled to transmit data, control signals and timing signals to the point sources 21, sensing elements 23 and pulse height analyzer 27 by signal lines 41- 43. The computer may comprise a known computer or plurality of computers and array processors adequate for image acquisition and image reconstruction processing. Commercial flow cytometers come with three basic flow configurations: namely, the cylindrical flow tube, the rectangular flow tube and the flow in air system. (See Shapiro, HM, Practical Flow Cvtometrv. 3rd ed., Wiley-Liss, 1995.) The preferred configuration is the cylindrical flow tube, because it is important to preserve optimal cylindrical geometry for the reconstruction algorithm to minimize any radial dependence due to the flow hardware (see FIG. 1). Moreover, the cylindrical flow tube may have uniformly thin walls relative to the cross-sectional area ofthe capillary tube.
Additionally, the triggering device may be located upstream from the reconstruction module to provide a timing signal to initiate then terminate data collection
as the cell optimally enters then emerges from the reconstruction cylinder. The triggering device may advantageously comprise a laser diode, CCD, PMT, a photodetector combination, a solid state photodetector and combinations ofthe foregoing elements. The triggering device has a threshold setting that senses the presence of a flowing cell, thus generating a trigger signal that, in conjunction with a known cell velocity, can be used to calculate when the downstream reconstruction cylinder may commence data collection for that particular cell of interest. Further, the time interval between the first and second trigger points corresponding to the entrance and exit of the cell into and out of the reconstruction cylinder, may be divided into equal or unequal increments during each of which additional projection data may be acquired by strobing the light source(s) 21 and reading out the sensor array(s) 23.
The velocity of flow needs to be controlled and measured accurately. This capability is provided for in high-end commercial systems that use velocities in the range of 1 meter/sec to 10 meters/sec. The best cell velocity will be determined by the speed of data collection and signal-to-noise considerations as discussed subsequently. The Reconstruction Module.
Referring now to FIG. 6, there shown schematically is an example of fan-beam projection rays within a reconstruction cylinder 20 as contemplated by an embodiment of the present invention. The pmpose of reconstruction cylinder is to provide a means of projecting light from a plurality of fixed point sources 21a - 21c, along a small circumference, into the cylindrical capillary tube. The photons emitted from the point sources have a known projection geometry, such as a fan or a cone shape, and pass through the capillary tube to be detected by an array of sensing elements 23a, 23b or 23c,
as the case may be, located along a larger circumference opposite a corresponding point source. While curved linear (ID) sensor arrays suitable for fan-beam transillumination are depicted for p poses of illustration, it is to be understood that straight linear (ID) sensor arrays or planar (2D) sensor arrays suitable for cone-beam illumination may be similarly employed. In this manner, a set of projection rays can be generated where the projection rays can be described as the straight line connecting the point source to an individual sensing element. The difference between the number of photons leaving the point source along a particular projection ray, such as ray 31, and the number of photons received at the particular sensing element is related to the number of photons lost or attenuated due to interactions with the cell and other contents ofthe flow tube along the projection ray path.
However, complications may arise from light scatter, photon energy shifts, imperfect geometry and poor collimation, and photons from different sources may arrive at a particular sensing element when multiple point sources are energized simultaneously.
With careful construction of the reconstruction cylinder, for example by judicious choice ofthe geometry for the pattern of point sources and their opposing detectors as described herein, and by proper timing or multiplexing of activation of the multiple point sources and readout of the sensor arrays, the photon contamination due to these issues can be minimized but not eliminated.
Photon contamination can be accounted for by calibration of the system, for example, with no cells present. That is, each light source may be illuminated in turn and its effects on each of the sensors can be measured, thereby providing offset data for use in normalizing the system. An additional calibration step may entail, for example, imaging latex polymer beads or other microspheres or oblate spheroids whose optical properties
are known and span the density range of interest for cellular imaging. Photons emitted from fluorescing probes may be differentiated from those originating at the point sources by the use of spectral bandpass filters at the detector as discussed subsequently. Light Source. Each source may have the same general characteristics, preferably:
• it may approximate a small circular point source,
• it may be bright with known spectral content,
• the photons emitted from the source may have a known geometry such as a cone-beam or a fan-beam. Each source creates data for one projection angle. A plurality of sources arranged along a helix whose axis is the center axis ofthe flow tube creates data from multiple projection angles through each successive plane (or reconstruction slice) as the cell flows through the module. Depending on the sensor geometry, several point sources could be arranged co- linearly on the same circumference such that the projections do not overlap at the sensor. A good sampling geometry can be achieved by placing sources equidistant along a helix of 180 degrees, though less angular coverage may be tolerable in some instances, and 360 degrees may be employed to improve the signal-to-noise ratio. The desired number of sources is a function of the needed resolution within each planar reconstruction (the x-y plane) or volumetric reconstruction. While a helical arrangement of point sources is used for illustration, it is to be understood that a variety of geometric patterns may be employed for the point source array. Further, the wavelength of the sources is selectable either by use of various diode or other lasers or by bandpass filtering of a white or other broadband source, for example a mercury or xenon arc lamp.
Now referring to FIG. 7, there shown schematically is an example of a top view of a reconstruction cylinder, as shown in FIG. 6, as contemplated by an embodiment of the present invention. A first point source 21a and sensor array 23a are shown with a cell with nucleus 19 flowing peφendicular to the page in a projection of the source trajectory which, in two dimensions, constitutes a circle of reconstruction 32, in which all projections, even though acquired in a temporally staggered fashion, are depicted as overlapping, and in which the whole cell is contained. A second point source 21b and second sensor array 23b are located about 30° around the helix. A third point source 21c and third sensor array 23c are located about 90° around the helix. Data collection is gated in synchrony with the cell velocity within a "thick" planar axial cross-section of the cell. The desired plane thickness is a function of the needed resolution in the z-direction. Typically, the resolution in the axial (z-direction) will be less than in the planar transaxial direction. Also, the best circle of reconstruction may be defined by the overlapping intersection of the projection fans having the point sources at their apexes and the width of the sensing arrays at their bases. It is desirable that the geometry of the reconstmction cylinder assures that the flowing cell cross section is contained entirely within the circle of reconstruction.
There are several options that can be employed to create optical point sources, such as: • a pinhole in front of a laser or other high intensity photon source,
• an optical fiber with a small cross-section,
• a short focal length lens in front of a photon source,
• an electron beam that irradiates a point on a phosphor surface (a form of CRT), and
• various combinations ofthe above.
The geometry is such that the closer the point source to the object of interest (the cell) the higher the magmfication due to the wider geometric angle that is subtended by an object closer to the source. Conversely, if the required resolution is known in advance of the system design, then the geometry can be optimized for that particular resolution. For background, those skilled in the art are directed to Blass, M, editor-in-chief, Handbook of Optics: Fiber Optics and Nonlinear Optics. 2nd ed., Vol. IV, Mcgraw-Hill, 2001. Referring now to FIG. 8, FIG. 8 schematically shows an example of a straight linear array 23 used in cell reconstruction as contemplated by an embodiment of the present invention. For example, given a cell cross section 12 and nucleus 19 contained within a 30-micron diameter circle of reconstruction and a desired resolution of 0.5 microns, then Nyquist sampling (i.e. over-sampling by a factor of two) dictates that at least 120 sensing elements 33 are required for each point source 21. The point source 21 at the apex and the linear array length 34 at the base form a triangle 35, such that the example 30-micron diameter cell fits within the triangle 35 as closely as possible to the point source 21. In this example, if each element of the (e.g. CCD) array is 20 microns wide and the array length is 2400 microns, then the center ofthe cell may be located about 100 microns (half the diameter of the capillary mbe) from the point source when the distance between the point source and the linear array is 8 millimeters, providing 80-fold magnification.
As a second example, consider a 30-micron diameter circle of reconstruction and a complementary metal oxide semiconductor (CMOS) sensing array in which the pixel element size is 4 microns. In this case the array may contain 120 elements for a width of 480 microns, and it may be positioned 1.6 mm from the point source when the distance between the point source and the cell is 100 microns, providing a 16-fold magnification. Sensing Elements
Each point source shall have a corresponding array of sensing elements such as CCDs in some straight or curved geometric arrangement opposite the point source to receive photon rays transmitted through the circle of reconstmction. Typically, the linear array may have its array of sensing elements centered on the line between the point source and the central flow axis, and may line up peφendicularly to the flow axis. It is possible to use 2D arrays where only a subset of each line of elements within the 2D array is read out for the reconstruction input. In a 2D array, each successive subset of elements may be staggered by the appropriate number of elements to align properly with each different point source along the helical arrangement of point sources.
For slice-by-slice fan-beam reconstruction using the example of the 30-micron reconstruction circle with 120 sensing elements per fan to obtain a resolution of 0.5 microns, a 2D array with 2000x2000 20-micron elements is sufficient for sensing 136, point sources arranged at 1 radial degree increments, where the average off-set between successive views is 300 microns, where that is equivalent to 15 sensing elements. (At the center ofthe array, the offset may be 140 microns, or 7 elements, while at the edges ofthe array, a 1 radial degree sweep between views may entail a considerably larger offset.) If groups of 15 rows ofthe sensor array were averaged to provide the projection data for one
slice, the z-resolution within the cell image may be 3.75 microns, whereas if 2 rows were averaged for each projection, the axial resolution in object space may be 0.5 microns, equivalent to the transaxial resolution.
In a preferred embodiment of the invention, the 2D array is curved along a cylindrical circumference that may be concentric with the reconstmction cylinder, so that the ray paths are all equal in length. For the case of a 30-micron reconstmction circle, a curved, 2D array that possessed only the elements required to oppose a helical locus of point sources may be a helical strip 120 elements wide by some multiple of 136 elements in height (length) for the example described above. Though planar or "thick" fan illumination is described for piuposes of the illustration above, it is to be understood that true, uncollimated cone-beam illumination may be employed in conjunction with 2D planar detectors, providing for 3D reconstruction using cone-beam algorithms. The 2D projection images may be analyzed directly to obtain, for example, information about the disease status or transformation state ofthe cell. For direct, volumetric cone-beam reconstruction, the illumination from a plurality of point sources is multiplexed in such a way that, given the geometric arrangement of the point sources and detectors, the cones of illumination from different point sources do not overlap on the sensor array.
Moreover, if the cell were flowing with a velocity of 1 meter/sec (or 1,000,000 microns/sec) and each element in the 2D array were 20 microns wide, then a line read-out every 20 microseconds may readily capture data within a 0.25-micron slice ofthe cell. For the case when 15 sensor rows are averaged to provide the data for a 3.75-micron slice,
readouts would have to occur every 300 microseconds. A significant improvement in reconstruction image quality is achieved using a larger 2D array.
One embodiment of the present invention especially suited for multispectral imaging of a number of transmitted or emitted wavelength bands may advantageously include two or more reconstruction modules arranged in series. Such multiple reconstruction cylinders may be separated by intervening sections of capillary mbe, and each module provides projection data adequate to produce a complete reconstructed image ofthe objects flowing through it. The point sources and/or sensor arrays for each of the several reconstruction modules may be optimized for a particular spectral band. For example, a first reconstmction module may employ intense white light illumination and unfiltered detection to provide a complete projection data set to reconstruct a map of object optical density, absoφtion or scattering coefficients, while a second reconstmction module may employ illumination, such as an argon-ion laser (488 nm), in a narrow spectral band centered around 495 nm to excite fluorescing probe labeling proteins for an immunofluorescence study in conjunction with filtered sensor arrays sensitive to the 520- nm emission to provide a second complete projection data set sufficient to map the concentration distribution of the labeled proteins by using emission reconstmction algorithms, as described subsequently. Yet a third reconstruction module may use narrowband illumination centered around 535 and or 342 nm to excite propidium iodide bound stoichiometrically to DNA and filtered sensor arrays to optimally detect the red (617-nm) emissions for studies of ploidy. It will be understood that the aforesaid examples are for illustrative puφoses, and that the method applies generally to any wavelength combinations for illuminating and sensing.
Image Reconstruction.
The most common and easily implemented reconstmction algorithms, known as filtered backprojection methods, are derived from a similar paradigm in computerized x- ray tomography (CT) using cone-beam and fan-beam geometry. (See the following references, for example, Kak, AC and Slaney, M. Principles of Computerized Tomographic Imaging. IEEE Press, New York, 1988, and Herman, G, Image Reconstruction from Projections: The Fundamentals of Computerized Tomography. Academic Press, New York, 1980.) These methods are based on theorems for Radon transforms with modifications that reflect the particular geometry of the source/detector configuration and the ray paths in the irradiating beam. However, in the case of clinical x- ray CT, for slice-by-slice acquisition, the human subject is usually held motionless while the x-ray source and detector arrays may move along an arc around the patient to collect data from multiple projection angles within a given slice. Then the human subject is repositioned along the z-axis and another slice of data is collected, etc. Alternatively, in the more modem clinical helical CT, the patient may be continuously translated in the z- direction while the source-detector assembly rotates continuously to provide helical projection data, which is then inteφolated to provide projections orthogonal to the patient z-axis. In flow optical tomography, the subject (a cell) is moved with constant velocity relative to the stationary sources and detector arrays wherein the plurality of source/detector systems acquire data in synchrony with specific gated time points along the cell velocity vector in a fashion that generates multiple projection angle data within a given slice or volume. For slice-by-slice scanning, the reconstruction algorithm will compute a 2D image of a plane peφendicular to the axis of motion, and the serial stacking
of multiple slices will generate the 3D picture of the subject where contrast is a function of the variations in the x-ray attenuation coefficient or optical density within the subject for CT or flow optical tomography, respectively. For volumetric, cone-beam scanning the reconstruction algorithm computes a 3D image of a volume within the cell or other object directly from planar transmission or emission optical projections, where the contrast is a function of the optical density and/or tagged probe density distribution, respectively, within the imaged object.
It may be desirable for either the transmission data to produce the cell density reconstruction or for the emission data to reconstruct the labeled probe distribution, or both, to employ image reconstruction algorithms other than filtered backprojection. The general class known as iterative reconstmction algorithms is more efficacious in some instances, especially for emission tomography or when it is possible, as in the instance of the current invention where the axial symmetry and tricompartmental nature ofthe object are known, to incoφorate a priori information into the reconstmction algorithm to improve the quality ofthe reconstruction(See, for example, Gilbert, P, "Iterative Methods for the Three dimensional Reconstmction of an Object from Projections," Journal of Theoretical Biology 36:105-17, 1972, and other references noted hereinabove).
Similarly, one method may advantageously use finite element modeling-based (FEM), statistical reconstmction algorithms. FEM algorithms are derived from linear transport theory in which the photon diffusion/migration equation is solved at all the boundaries of the elements to produce a two- or three dimensional map of some combination ofthe absoφtion, scattering, refractive index and anisotropy factor properties of the imaged object. Examples of such methods are taught in Paulsen, KD and Jiang, H,
"Spatially Varying Optical Property Reconstmction Using a Finite Element Diffusion Equation Approximation", Medical Physics 22(691-701) 1995, Hampel, U and Freyer, R, "Fast Image Reconstmction for Optical Absoφtion Tomography in Media with Radially Symmetric Boundaries", Medical Physics 25 (1):92-101, 1998, and Jiang, H, Paulsen, KD, and Osterberg, UL, "Frequency-domain Near-infrared Photo Diffusion Imaging: Initial Evaluation in Multitarget Tissuelike Phantoms", Medical Physics 25(2): 183-93, 1998. Chromatic Separation.
If a polychromatic point source is used (e.g., white light) then different chromatic stains (e.g. chromaphors) can be utilized to distinguish a number of molecular probes and stmctural features within a given cell. Here, serial bandpass filters at the source or sensing array (or both) separate the wavelength data and allow the reconstmction and spatial localization of the individually stained molecules. A more robust method for imaging multiple probes involves an intense white light source and simultaneous collection of multiple filtered bandwidths in the sensor arrays thus allowing the image reconstmction algorithms to compute spatial image slices for each chromaphor. These may be displayed as colored images. Fluorescence, Phosphorescence, Chemiluminescence and Nano-Particle Emission
As a special case ofthe flow optical tomography system, certain molecular probes can be tagged with a "reporter" that emits light of a different (longer) wavelength when stimulated by the primary source of photons. The secondary emission from the reporter can be filtered with standard optical filters to separate the primary source photons from the secondary emission photons. However, the secondary emission photon image reconstruction algorithm is further complicated, because the secondary photons do not
necessarily arise in a direct ray path from the point source. If it is assumed that the secondary photons radiate from the secondary point source in a uniform spherical pattern, then the intensity ofthe secondary photons reaching any sensing element will be a simple function of distance to the sensing element. A further refinement may account for the non- spherical distribution of photons from the secondary source by providing a model of the spatial distribution of secondary photons relative to the point source and within the reconstmction slice. Either method will provide a means to calculate the location of the secondary source in the reconstmction slice or volume. Collimation between the imaged object and the detector array(s) will improve the image reconstmction. If the primary photon intensities and the secondary photon intensities are measured simultaneously by optical filtration, the high resolution density reconstmction from the primary photon intensities can be superimposed upon or fused with the secondary source reconstmction such that image moφhology along with localized probe concentration is available in a single reconstructed image. Depending on intensity, signal-to-noise and on the ability to filter or produce narrow bandwidths of photons at the source and/or sensors, it may be advantageous to utilize multiple secondary sources each corresponding to a different tagged molecular probe.
US Patent No. 6,201,628 entitled "High Throughput Optical Scanner", issued March 13, 2001, to Basiji, et al. discloses a scanning apparatus provided to obtain automated, rapid and sensitive scanning of substrate fluorescence, optical density or phosphorescence. The scanner uses a constant path length optical train, which enables the combination of a moving beam for high speed scanning with phase-sensitive detection for noise reduction, comprising a light source, a scanning mirror to receive light from the light
source and sweep it across a steering mirror, a steering mirror to receive light from the scanning mirror and reflect it to the substrate, whereby it is swept across the substrate along a scan arc, and a photodetector to receive emitted or scattered light from the substrate, wherein the optical path length from the light source to the photodetector is substantially constant throughout the sweep across the substrate. The optical train can further include a waveguide or mirror to collect emitted or scattered light from the substrate and direct it to the photodetector. For phase-sensitive detection the light source is intensity modulated and the detector is connected to phase-sensitive detection electronics. A scanner using a substrate translator is also provided. For two dimensional imaging the substrate is translated in one dimension while the scanning mirror scans the beam in a second dimension. For a high throughput scanner, stacks of substrates are loaded onto a conveyor belt from a tray feeder. US Patent No. 6,201,628 is incoφorated herein by reference.
The invention has been described herein in considerable detail in order to comply with the Patent Statutes and to provide those skilled in the art with the information needed to apply the novel principles of the present invention, and to construct and use such exemplary and specialized components as are required. However, it is to be understood that the invention may be carried out by specifically different equipment, and devices and reconstmction algorithms, and that various modifications, both as to the equipment details and operating procedures, may be accomplished without departing from the tme spirit and scope ofthe present invention. What is claimed is:
Claims (66)
1. A flow optical tomography method for imaging and analysis of microscopic objects, the method comprising the steps of:
(a) injecting at least one object into an injection mbe (3); (b) controlling the flow ofthe at least one object through a capillary mbe (2) such that the at least one object elongates along an axis of flow and moves proximately along a central axis (9) of the capillary mbe (2); (c) sampling with at least one optical point source (21), located around a circumference of the capillary mbe (2), in conjunction with at least one opposing optical sensor (23) disposed opposite the at least one optical point source (21) at a distance from the capillary mbe (2) such that there is no focal plane within the at least one object, and where multiple projection angles through the at least one object are sampled as it flows past the at least one optical point source (21) and at least one opposing optical sensor (23); and (d) generating a series of timing signals (28, 29), such that each timing signal (28, 29) coincides with a specific position along the axis (9) in the z-direction ofthe at least one object, so as to generate a set of timed optical projections through the at least one object.
2. The method of claim 1 further comprising the step of reconstmcting the set of timed optical projections to form a two dimensional (2D) slice.
3. The method of claim 1 further comprising the step of reconstmcting the set of timed optical projections to form a three dimensional (3D) volume.
4. The method of claim 2 further comprising the step of combining sequential 2D slices to produce a three dimensional (3D) image ofthe at least one object.
5. The method of claim 1, wherein the optical projections comprise two dimensional (2D) optical projections, further comprising the step of producing a three dimensional (3D) image ofthe at least one object from two dimensional (2D) optical projections.
6. The method of claim 1 further comprising the step of creating laminar flow within the capillary mbe (2) such that the at least one object moves with a constant velocity (N).
7. The method of claim 1 wherein the at least one object is a cell (1).
8. The method of claim 5 further comprising the step of using the 3D image to yield quantitative measures of microscopic structures.
9. The method of claim 8 wherein the microscopic stmctures comprise sub-cellular stmctures.
10. The method of claim 5, wherein the at least one object includes a cell (1) having at least one tagged molecular probe therein, further comprising the step of using the 3D image to determine a location and amount ofthe at least one tagged molecular probe.
11. The method of claim 2, wherein the at least one object includes a cell (1) having at least one molecular probe therein, where the molecular probe provides molecular probe information, the method further comprising the step of combining the 2D slice and the molecular probe information so as to ascertain any association between particular sub-cellar stmctures and the at least one molecular probe.
12. The method of claim 1, wherein the at least one object includes a cell (1), the method further comprising the step of operating in a circle of reconstruction for cell imaging and analysis, such that the space being sampled by projections is modeled as consisting of at least three compartments:
(a) the fluid outside the cell (1),
(b) the cell cytoplasm (18), and (c) the cell nucleus (19).
13. The method of claim 12 further comprising the steps of:
(a) computing boundary surfaces including a cell wall (12) and a nuclear wall (13) if certain ones of the at least one molecular probe bind only to surfaces of the cell wall (12) and the nuclear wall (13); and (b) otherwise characterizing the surfaces ofthe cell wall (12) and the nuclear wall (13) as transition surfaces between the three different compartments.
14. The method of claim 12 further comprising the steps of:
(a) measuring the relative over or under expression of a gene product in the cell cytoplasm (18) relative to the nucleus (19); and (b) normalizing for non-bound probes in the background suspension fluid.
15. The method of claim 14 further comprising the step of using a tagged antibody probe to assess at least one of a disease state and a transformation state of the cell (1) if the gene product is a protein.
16. The method of claim 14 further comprising the step of using a nucleic acid probe to assess at least one of a disease state and a transformation state of the cell (1) if the gene product is a protein.
17. A flow optical tomography system for imaging and analysis of microscopic objects, comprising: (a) a flow cytometer including a capillary mbe (2);
(b) at least one reconstruction cylinder (20) positioned around the capillary mbe (2); and
(c) a triggering device (25, 26, 27), located to view the at least one object flowing through the capillary tube (2), for creating a trigger signal (28,29) for at least one object, where the trigger signal (28, 29) is received by the at least one reconstmction cylinder (20), and where the at least one reconstmction cylinder (20) responds to the trigger signal (28, 29) by producing signals representing a projection image about the at least one object and the signals are processed to provide three dimensional information about the at least one object .
18. The flow optical tomography system of claim 17, where the at least one object moves with a velocity (V) through the capillary mbe (2), and wherein the at least one object comprises a cell (1) having wall of cell cytoplasm and a wall of cell nucleus (13), further, during the course of flowing through the capillary mbe (2), the cell (1) passes through a plurality of reconstruction planes, a planar slice through the wall ofthe cell nucleus (13) lies within each reconstmction plane, where, a distance (d) between reconstmction planes is typically less than 10 microns and a point within each cell (1) coincides with each reconstmction plane at time intervals (t), where the time intervals are described according to the relationship: t = d ÷ V
19. The flow optical tomography system of claim 18, where the cells (1) are labeled with at least one tagged molecular probe for disease diagnosis.
20. The flow optical tomography system of claim 17, further comprising: (a) means for controlling the velocity (V) of the at least one object flowing proximately along an axis;
(b) means for locating two dimensional (2D) planes of reconstmction along an axis (9) of the at least one object to create a three dimensional (3D) image of the at least one object; and
(c) means (27, 40) for correctly locating the position ofthe at least one object in the reconstmction cylinder (20) to create a three dimensional (3D) image of the cell (1) from a set or plurality of sets of two dimensional (2D) projection data.
21. The system of claim 17 wherein the at least one reconstmction cylinder comprises: (a) a helix of point sources (21) disposed at a predetermined helical pitch, where each point source (21) generates a beam of photons (22), where the beam (22) has a fan or cone shape, where the at least one object moves past the helix of point sources to generate multiple projections at different angular orientations through the at least one object; (b) a locus of point sources (21) disposed in a geometric pattern around the at least one cylinder (20) concentric with a capillary mbe axis (9); and (c) where the point sources(21) emit photons that pass as radiating projections through the at least one object and are detected by at least one sensor (23) opposite the point sources (21).
22. The system of claim 21 wherein a plurality of reconstruction cylinders (20) are arranged in series, and where the optical sources (21) illuminating the at least one object passing through the flow mbe may emit at wavelengths spanning the electromagnetic spectrum from x-ray to far infrared.
23. The system of claim 22 wherein the sources within and/or between reconstmction cylinders (20) differ in their emission spectra.
24. The system of claim 23 wherein the emission spectra comprise narrow band spectra centered around the excitation maxima of immunofluorescence dyes and tags.
25. The system of claim 22 wherein a plurality of reconstmction cylinders (20) are arranged in series, and where the light sensor arrays (23) are spectrally bandpass filtered for sensitivity to the wavelengths emitted by the fluorophores employed for at least one of immunofluorescence studies and ploidy studies.
26. The system of claim 22 wherein the plurality of reconstmction cylinders (20) are arranged in series with intervening sections of capillary mbe (2).
27. The system of claim 22 wherein the range of the emitted wavelengths span the electromagnetic spectrum from 10 Angstroms to 2000 microns.
28. The system of claim 17 wherein a plurality of point sources (21) are arranged along a geometric pattern on the capillary mbe (2) such that each point in the at least one object is sampled from a multitude of angles as it passes through the array of point sources (21).
29. The system of claim 28 wherein the geometric pattern comprises a helical pattern.
30. The system of claim 29 where the point sources (21) cover any angular extent of the circumference and are spaced in equiangular increments along at least 180 degrees.
31. The system of claim 17 wherein the capillary mbe (2) comprises uniformly thin walls relative to the cross-sectional area ofthe capillary flow.
32. The system of claim 17 wherein the triggering device (25, 26) is located upstream from the reconstmction module to provide a timing signal to initiate and subsequendy terminate data collection as the at least one object enters then emerges from the reconstruction cylinder.
33. The system of claim 17 wherein the triggering means comprises elements selected from the group consisting of a laser diode, CCD, PMT, a solid state photodetector and combinations ofthe forgoing elements.
34. The system of claim 17 wherein the triggering means generates a trigger signal that, in conjunction with the at least one object velocity (V), is used to calculate when the downstream reconstmction module can commence data collection for the at least one object of interest.
35. The system of claim 34 wherein the triggering means (25, 26, 27) generates a trigger signal (28, 29) that, in conjunction with the at least one object velocity (V), is used to calculate a point in time for the downstream reconstmction module to proceed to acquire multiple sets of projection data at temporal increments based on the set of upstream trigger signals (28, 29).
36. The system of claim 17 wherein the capillary mbe (2) is constmcted to produce velocities in the range of 1 meter/sec to 10 meters/sec.
37. The system of claim 17 wherein the reconstmction cylinder (20) produces projection rays from a plurality of fixed point sources (21) into the capillary tube (2), and photons emitted from the point sources have a selected projection geometry such that there is no focal plane within the object.
38. The system of claim 37 wherein the selected projection geometry is selected from the group consisting of a cone shape and a fan shape.
39. The system of claim 37 wherein the projection rays pass through at least one object to be detected by at least one array of sensing elements.
40. The system of claim 39 wherein:
(a) the at least one array of sensing elements (23) is positioned opposite a corresponding point source (21) and where the arrays (23) are arranged in any geometric pattern; and
(b) the at least one array of sensing elements (23) has optical bandpass filters, where the spectral bands passed are different for the sensing arrays either within or between the plurality of reconstmction modules (20).
41. The system of claim 17 wherein offset data is provided for normalizing the system.
42. The system of claim 41 wherein the system is calibrated by i) acquiring images in the absence of any at least one object in the flow mbe, and ii) acquiring images of at least one object of known optical properties.
43. The system of claim 42 where the calibration data is reconstructed.
44. The system of claim 42 wherein the at least one object of known optical properties is selected from the group consisting of latex microspheres, polymer microspheres, and oblate spheroids.
45. The system of claim 37 wherein each point source comprises a circular point source.
46. The system of claim 37 wherein a circle of reconstmction is defined by radially overlapping projection fans from the point source at the apex and the width of the sensing array at the base.
47. The system of claim 37 wherein the point sources comprise a point source device selected from the group consisting of: (a) a pinhole in front of a laser;
(b) an optical fiber;
(c) a short focal length lens in front of a photon source;
(d) an electron beam that irradiates a point on a phosphor surface; and (e) a high intensity photon source; and
(f) any combination ofthe above elements (a) through (e).
48. The system of claim 37 wherein the array of sensing elements comprise elements selected from the group consisting of charge coupled devices (CCDs), photodiodes, CMOS, CdZnTe, Mgl sensors, solid state sensors, a photon-sensitive array of elements in any geometric arrangement, including a linear arrangement.
49. The system of claim 48 wherein the array of sensing elements are centered on the line between the point source and the central flow axis.
50. The system of claim 49 wherein the array of sensing elements line up peφendicularly to the flow axis.
51. The system of claim 29 further comprising a plurality of fixed point sources having successive subsets of elements staggered to align properly with each different point source along the helical arrangement of point sources (21 ).
52. The system of claim 29 wherein the array of sensing elements (23) is curved along a cylindrical circumference that is concentric with the reconstmction cylinder (20).
53. The system of claim 17 wherein the reconstruction cylinder (20) provides image signals that are reconstructed using filtered backprojection algorithms where the algorithm computes a two dimensional (2D) image of a slice peφendicular to the axis of motion, and the serial stacking of multiple slices generates a three dimensional (3D) image ofthe at least one object where contrast is a function ofthe variations in optical density within the at least one object.
54. The system of claim 17 where chromaphors are used to distinguish a number of molecular probes and stmctural features within a given cell (1).
55. The system of claim 17 fiirther comprising serial bandpass filters coupled to the reconstmction cylinder to separate wavelength data and allow the reconstmction and spatial localization ofthe individually stained molecules.
56. The method of claim 1 further comprising the step of illuminating the at least one object with an intense white light source and simultaneously collecting multiple filtered bandwidths.
57. The method of claim 1 further comprising the steps of
(a) tagging molecular probes with a reporter that emits light of a different wavelength when stimulated by the primary source of photons; and
(b) filtering the secondary emission from the reporter to separate the primary source photons from the secondary emission photons.
58. The system of claim 17 wherein the reconstmction cylinder (20) is produced by microfabrication techniques.
59. A flow optical tomography system for imaging and analysis of microscopic objects, the method comprising: a pulse height analyzer (27), a source of photons and a photon sensor (23), where the source of photons and the photon sensor (23) work together with the pulse height analyzer (27) to operate as a triggering device, where the pulse height analyzer (27) provides a first trigger point (28) for the beginning of a the at least one object, and a second trigger point (29) for the end of the at least one object to create a corresponding trigger signal delivered to a reconstruction cylinder for the puφose of synchronizing object velocity (V) and position with each projection slice.
60. The method of claim 3, wherein the cell (1) includes at least one molecular probe, where the molecular probe provides molecular probe information, the method further comprising the step of combining the 3D volume and the molecular probe information so as to ascertain any association between particular sub-cellar structures and the at least one molecular probe.
61. The method of claim 4, wherein the cell (1) includes at least one molecular probe, where the molecular probe provides molecular probe information, the method further comprising the step of combining the 3D image and the molecular probe information so as to ascertain any association between particular sub-cellar structures and the at least one molecular probe.
62. The method of claim 5, wherein the cell (1) includes at least one molecular probe, where the molecular probe provides molecular probe information, the method further comprising the step of combining the 3D image and the molecular probe information so as to ascertain any association between particular sub-cellar structures and the at least one molecular probe.
63. The method of claim 7 further comprising the step of processing and analyzing the projection images directly to assess the disease status or transformation state of a cell (1).
64. The system of claim 20 further comprising a means for processing and analyzing a set of projection images directly to assess the disease status or transformation state of a cell (1).
65. The system of claim 37 wherein a volume of reconstmction is defined by radially overlapping projection cones from the point source at the apex and the width of the sensing array at the base.
66. The system of claim 17 wherein the reconstmction cylinder (20) provides image signals that are reconstructed using filtered backprojection algorithms where the algorithm computes a two dimensional (2D) image of a slice peφendicular to the axis of motion, and the serial stacking of multiple slices generates a three dimensional (3D) image of the at least one object where contrast is a function of variations in probe emission density within the at least one object.
Applications Claiming Priority (2)
Application Number | Priority Date | Filing Date | Title |
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US60/279,244 | 2001-03-28 | ||
US09/927,151 | 2001-08-10 |
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AU2002303160A1 AU2002303160A1 (en) | 2003-04-03 |
AU2002303160B2 true AU2002303160B2 (en) | 2007-03-08 |
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