Classifications

• • G—PHYSICS
  • G02—OPTICS
  • G02B—OPTICAL ELEMENTS, SYSTEMS OR APPARATUS
  • G02B21/00—Microscopes
  • G02B21/36—Microscopes arranged for photographic purposes or projection purposes or digital imaging or video purposes including associated control and data processing arrangements
  • G02B21/365—Control or image processing arrangements for digital or video microscopes
• • G—PHYSICS
  • G02—OPTICS
  • G02B—OPTICAL ELEMENTS, SYSTEMS OR APPARATUS
  • G02B21/00—Microscopes
  • G02B21/18—Arrangements with more than one light path, e.g. for comparing two specimens
• • 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
  • G02B21/0056—Optical details of the image generation based on optical coherence, e.g. phase-contrast arrangements, interference arrangements
• • G—PHYSICS
  • G02—OPTICS
  • G02B—OPTICAL ELEMENTS, SYSTEMS OR APPARATUS
  • G02B21/00—Microscopes
  • G02B21/02—Objectives
• • G—PHYSICS
  • G02—OPTICS
  • G02B—OPTICAL ELEMENTS, SYSTEMS OR APPARATUS
  • G02B21/00—Microscopes
  • G02B21/24—Base structure
  • G02B21/248—Base structure objective (or ocular) turrets
• • G—PHYSICS
  • G02—OPTICS
  • G02B—OPTICAL ELEMENTS, SYSTEMS OR APPARATUS
  • G02B21/00—Microscopes
  • G02B21/24—Base structure
  • G02B21/26—Stages; Adjusting means therefor

Definitions

• TITLE OF THE INVENTION Module intended to be associated with a microscope, assembly of a microscope and such a module
• the invention relates to a module intended to be associated with a microscope for full-field optical coherence tomography microscopic imaging of at least one sample.
• the invention also relates to a set of such a module and a microscope.
• organoid technology makes it possible to overcome at least in part the difficulties linked to the creation of three-dimensional human tissue replicating in particular physiological conditions in vivo.
• this organoid technology makes it possible to produce indefinitely material that can be described as “human” without ethical constraints and could therefore, ultimately, lead to the reduction or even replacement of studies on animal models.
• Organoids can thus be used for disease modeling, to carry out effectiveness tests of new treatments (genes, pharmaceuticals, etc.), for transplantation, etc.
• organoids technology noids has become mature, it still proves complicated to be able to carry out control imaging with sufficient precision, which is non-destructive, to ensure the proper functioning of these organoids.
• Optical coherence tomography imaging (better known by the acronym OCT for “Optical Coherence Tomography”) makes it possible to acquire images with greater precision.
• OCT Optical Coherence Tomography
• full-field optical coherence tomography imaging is based on the acquisition of signals originating from the interference between a signal of retrodifference flared by a sample when it is illuminated by a source with a signal reference light emitted by this same source.
• Document FR 2 817 030 describes an example of an interference microscopic imaging system with full-field optical coherence.
• the invention aims in particular to enable full-field optical coherence tomography microscopic imaging of at least one sample which is easy to implement.
• a module intended to be associated with a microscope for full-field optical coherence tomography microscopic imaging of at least one sample, the module comprising an interference device comprising an element non-polarizing beam splitter, the device further comprising a reflection surface, the device thus being able in service to allow the production of at least one interference between:
• the non-polarizing beam splitter element thus making it possible in use to form two arms, when illuminated by the source, namely a “ reference arm” associated with the reflection surface and an “object arm” associated with the sample, the device further comprising:
• a first adjustment unit arranged upstream of the non-polarizing beam splitter element to be able to modify in service a lighting arm of the non-polarizing beam splitter element, and/or - at least a second adjustment unit arranged between the beam splitter element and the reflection surface to be able to modify the reference arm in service.
• the invention can be coupled to an existing microscope to be able to carry out full-field optical coherence tomography microscopic imaging. It is enough to associate the invention with the microscope then to use the adjustment unit(s) to ensure interference between the reference waves and the object waves.
• the second unit is adjusted so that the reference arm is identical to the object arm, that is to say that the optical paths in the two arms are equal (up to the spatial coherence length of the source) when the microscope is coupled to the module.
• the first unit is adjusted so as to align, in use, a working axis of the module (i.e. the axis along which the majority of light rays propagating on the object arm exit the module to reach the microscope) with a propagation axis of the source (i.e. the axis along which the majority of light rays generated by the source propagate).
• a working axis of the module i.e. the axis along which the majority of light rays propagating on the object arm exit the module to reach the microscope
• a propagation axis of the source i.e. the axis along which the majority of light rays generated by the source propagate.
• the invention facilitates access to full-field optical coherence tomography microscopic imaging.
• the associated microscope can be a microscope for which other optical modules [differential interference contrast module better known by the English acronym DIC module (for Differential Interference Contrast), coherent anti-Stokes Raman scattering module more known by the acronym CARS module (for Coherent Anti-Stokes Raman Scattering), second harmonic generation module better known by the English acronym SHG module (for Second Harmonie Generation), third harmonic generation module better known as The English acronym for THG module (for Third Harmonie Generation), Raman module, one or two photon fluorescence module, etc.] have already been developed.
• DIC module for Differential Interference Contrast
• CARS module for Coherent Anti-Stokes Raman Scattering
• second harmonic generation module better known by the English acronym SHG module (for Second Harmonie Generation)
• third harmonic generation module better known as The English acronym for THG module (for Third Harmonie Generation)
• Raman module one or two photon fluorescence module, etc.
• the module of the invention can thus easily be coupled to these modules of the prior art, which makes it possible to enrich the possibilities for imaging the sample.
• the associated microscope may be a microscope for which accessories have already been developed so that by connecting to such a microscope, the invention makes it possible to benefit from the accessories of the microscope.
• the invention can be connected to a standard microscope and thus advantageously allows access to numerous options already developed for this microscope.
• the invention makes it possible to implement different types of full-field optical coherence tomography microscopic imaging.
• the invention can thus also make it possible to carry out full-field optical coherence tomography imaging (better known by the English acronym FFOCT for “Full-Field Optical Coherence Tomography”) - that is to say, i.e. so-called “static” imaging - as dynamic full-field optical coherence tomography imaging (better known by the acronym D-FFOCT for “Dynamic FFOCT”).
• FFOCT Full-field optical coherence Tomography
• D-FFOCT dynamic full-field optical coherence tomography imaging
• D-FFOCT Dynamic FFOCT
• the invention makes it possible, for example, to be able to look at elements present in a sample (static imaging) as well as elements which make up a tissue of one of said structures of the same sample (dynamic imaging).
• the elements can for example be cells, structures and in particular subcellular structures such as nuclei, mitochondria
• the invention can therefore be used for numerous applications and/or according to different operating modes (static imaging or dynamic imaging).
• the invention thus proves to be particularly modular.
• the invention makes it possible to reduce the cost of optical coherence tomography microscopic imaging since the invention is grafted onto an existing microscope.
• reference arm means the part of the module located between the reflection surface and the non-polarizing beam splitter element (a light ray can thus propagate in said reference arm following a given optical path) .
• object arm means the part of an assembly formed by the module and the microscope located between the sample and the non-polarizing beam splitter element (a light ray can thus propagate in said object arm following a given optical path).
• lighting arm means the part of an assembly formed by the module and the microscope located between the source and the non-polarizing beam separator element (a light ray can thus propagate in said arm object following a given optical path).
• modification of a propagation characteristic for example a modification of a relative position of a frame of the module with respect to the source, for example to modify the relative position of the frame with respect to the source. with respect to the axis of propagation of the source and/or the incidence with which the light rays generated by the source reach the non-polarizing beam splitter element.
• the first adjustment unit comprises at least two reflection surfaces, at least one of said reflection surfaces being movable with respect to a frame of the module.
• the module includes an objective associated with the reference arm, the second adjustment unit comprising at least one additional reflection surface and at least one member for moving said objective with respect to a frame of the module.
• the additional reflection surface and also movable in relation to a module frame.
• the movement member is configured to move the objective at least in a plane parallel to the plane in which the first reflection surface extends.
• the source is part of the module.
• the module includes an acquisition device adapted to acquire at least one signal resulting from interference between the reference waves and the object waves.
• the interference device comprises an optic arranged between the separator element and an output of the module intended to be coupled at least optically to the microscope.
• the invention also relates to an assembly comprising a microscope and a module as mentioned above.
• the microscope includes a turret, the module being arranged in one of the turret compartments.
• the assembly includes an incubator carried by a microscope stage.
• FIG. 1 is a schematic view of an assembly of a microscope and a module according to a particular embodiment of the invention.
• Figure 1 schematically illustrates a set of full-field optical coherence tomography microscopic imaging of at least one sample according to a particular embodiment of the invention.
• the assembly 1 thus comprises at least one microscope 2 and a module 3 connected to the microscope 2.
• module 3 is shaped to be able to be arranged in one of the lockers of the row of lockers of the microscope 2, row forming a turret.
• module 3 is very simply coupled to said microscope 2 (mechanically as well as optically) by simple insertion of module 3 into microscope 2.
• the microscope 2 is shaped so as to present at least one optical output facing at least one row so that the module inserted in said row is de facto optically coupled to the microscope 2.
• Microscope 2 is for example an inverted microscope.
• an inverted microscope is a microscope in which a sample is observed from below.
• Microscope 2 is advantageously a conventional microscope.
• Microscope 2 is for example a 1X83 marketed by the company Olympus.
• the microscope 2 comprises a stage intended to carry a sample to be observed, the stage being movable in translation with respect to a frame of the microscope 2 along at least two axes of translation.
• the microscope also includes a turret allowing the insertion of modules to interact with the microscope 2.
• the module 3 comprises an interference device 4 which here comprises a source 5 and a reflection surface 6, the interference device 4 thus being able, in service, to produce optical interference between: reference waves obtained by reflection of the light emitted by the source 5 on the reflection surface 6, and • object waves obtained by backscattering the light emitted by said source 5 on the sample.
• an interference device 4 which here comprises a source 5 and a reflection surface 6, the interference device 4 thus being able, in service, to produce optical interference between: reference waves obtained by reflection of the light emitted by the source 5 on the reflection surface 6, and • object waves obtained by backscattering the light emitted by said source 5 on the sample.
• the source 5 is a source that is spatially incoherent or of short spatial coherence length (i.e. for example in a range of 0.5 to 120 micrometers or for example in a range of 0.8 to 100 micrometers or for example a range of 1 to 20 micrometers).
• the source 5 is for example a halogen lamp or a light-emitting diode (better known by the acronym LED) or even a block formed of a coherent source (the coherent source being for example a laser) and a structure crossed by the rays at the output of the coherent source, a structure making it possible to make said rays spatially incoherent at the output of the structure (and therefore of the block).
• the structure is for example provided with a multimode type cavity, a multimode fiber, a hexagonal rod, etc.
• the reflection surface 6 is flat.
• the reflection surface 6 is for example a mirror.
• the assembly 1 also comprises here an acquisition device 7.
• the acquisition device 7 is part of module 3.
• the acquisition device 7 allows the acquisition of at least one signal resulting from the interference between reference waves and object waves.
• the acquisition device 7 comprises an optical sensor.
• the optical sensor is preferably an optical sensor with semiconductors complementary to the metal oxide (better known by the English term CMOS for Complementarity metal-oxide-semiconductor).
• the optical sensor is chosen to acquire images at a high rate. This allows you to see following, if desired, a dynamic of movements within the sample when it includes at least one living cell.
• the optical sensor is capable of acquiring images at a frequency greater than 100 Hertz and preferably greater than 200 Hertz and preferably greater than 400 Hertz.
• the optical sensor is chosen to acquire images with a high signal-to-noise ratio. This allows the optical sensor to be sensitive even to very small living structures and/or to even very small movements.
• the optical sensor is capable of acquiring images with a signal-to-noise ratio greater than 500 and preferably greater than 800 and preferably greater than 1000.
• the optical sensor is a camera and for example a CMOS camera and for example a Q-2A750 camera or a Q-2HFW camera both marketed by the company Adimec.
• the assembly 1 also comprises here a device for processing the signal 8 emitted by the acquisition device 7 to, for example, generate an image of at least part of the sample.
• the signal processing device 8 is external to the module 3.
• the signal processing device 8 comprises at least one processing unit such as a processor.
• the signal processing device 8 includes, for example, a computer.
• assembly 1 comprises an incubator 9 for a microscope.
• the incubator 9 is for example arranged in the microscope 2 so as to be carried by the stage of the microscope 2, the sample being placed directly in the incubator 9.
• the incubator 9 is preferably portable so that it can be temporarily attached to the microscope 2.
• the incubator 9 makes it possible to facilitate the study of samples comprising at least one living cell. Indeed, the incubator 9 makes it possible to keep such samples alive over several days or even several weeks.
• the incubator 9 is shaped to be able to receive multi-well plates.
• the incubator 9 is equipped with temperature control within the incubator 9.
• the incubator 9 is equipped with a control of the presence of at least one gas in the incubator.
• the incubator is equipped with a control of the presence of carbon dioxide in the incubator and/or the presence of nitrogen in the incubator and/or the presence of oxygen in the incubator.
• the incubator 9 is preferably configured to maintain the sample at a given temperature and for example at a temperature substantially equal to 37 degrees Celsius (for example human cells, primates, pork, etc.).
• the incubator 9 is configured to allow the oxygenation of the sample (in particular by a supply of a nitrogen and dioxygen mixture and an evacuation of carbon dioxide) this oxygenation being ensured by at least the control of the rate of carbon dioxide in the incubator.
• the incubator 9 is configured to allow the humidity level of the sample to be managed so that the sample does not dehydrate.
• the incubator 9 is equipped with a sensor making it possible to ensure that the humidity level in the incubator 9 is between 70 and 100%.
• incubator 9 is advantageously here a conventional incubator.
• incubator 9 is an H201-K incubator marketed by the company Okolab.
• the interference device 4 comprises a frame carrying a base which is immobile with respect to the frame.
• Said base carries a non-polarizing beam splitter element 10 (better known by the English acronym NPBS for Non-Polarizing Beamsplitters).
• the separator element 10 is for example a non-polarizing separator cube, a non-polarizing separator blade, etc.
• the source 5 is intended to illuminate the separator element 10. However, the source 5 does not directly illuminate the separator element 10. The source 5 is thus offset from the separator element 10 and the base. The source 5 is thus fixed to a portion of the frame.
• the interference device 4 comprises a first adjustment unit 11 via which the source 5 will illuminate the separator element 10.
• the first adjustable unit 11 comprises at least one reflection surface.
• the first adjustment unit 11 comprises at least two reflection surfaces 12, 13 which are mounted opposite each other.
• the reflection surfaces 12, 13 are planar.
• the reflection surfaces 12, 13 are for example mirrors.
• the first adjustment unit 11 is arranged so that in use the source 5 directly illuminates one of the reflection surfaces 12 which reflects the light towards the other of the reflection surfaces 13 which in turn reflects the light towards the separator element 10 so as to illuminate it.
• At least one and preferably both reflection surfaces 12, 13 are mounted movable with respect to the frame.
• the first adjustment unit 11 is designed such that the two reflection surfaces 12, 13 can be moved relative to the frame independently of each other.
• at least one of the reflection surfaces and preferably the two reflection surfaces 12, 13 can pivot relative to the frame.
• the first adjustment unit 11 comprises a first kinematic mount carrying the reflection surface 12 (and making it possible to move said reflection surface 12 with respect to the frame) and a second kinematic mount carrying the reflection surface 13 ( and allowing said reflection surface 13 to be moved with respect to the frame). Thanks to the movements of the reflection surfaces 12, 13, it is for example possible to modify the optical path of the rays generated by the source 5 to the separator element 10.
• the interference device 4 comprises a first optic 14 arranged upstream of the first adjustment unit 11 (the notions of “upstream” and “downstream” being understood according to the direction of circulation of the light) between the source 5 and the first adjustment unit 11.
• the first optic 14 makes it possible in particular to reduce the divergence of the rays generated by the source 5. This limits a loss of power of the light radiation generated by the source 5.
• the first optic 14 is for example a single lens, a single doublet or a pair of lenses or a pair of doublets. If the first optics 14 is a pair of doublets, the first optics 14 is composed for example of a first achromatic doublet (i.e. a set of an achromatic converging lens and a plane lens corrected to infinity upstream) and a second achromatic doublet (i.e. a set of an achromatic converging lens and a plane lens corrected to infinity downstream), the second doublet being arranged downstream of the first doublet.
• the flat faces of the lenses are respectively turned towards the source 5 and the adjustment unit 11.
• the interference device 4 comprises a second optic 15 arranged downstream of the first adjustment unit 11 between the first adjustment unit 11 and the separator element 10.
• the second optic 15 is for example a lens, a doublet, etc.
• the second optic 15 is for example an achromatic doublet comprising an achromatic converging lens and preferably an achromatic converging lens having a flat face which is the one facing the first adjustment unit 11.
• the interference device 4 comprises a first diaphragm 16 arranged upstream of the first adjustment unit 11 between the source 5 and the first adjustment unit 11.
• the first diaphragm 16 is arranged downstream of the first optics 14 between the first optics 14 and the first adjustment unit 11.
• the first diaphragm 16 is for example an aperture diaphragm.
• the first diaphragm 16 is arranged in a focal plane of the second doublet of the first optics 14 and preferably in the image focal plane of the second doublet of the first optics 14.
• first optics 14 images the source 5 at the image focal plane of said second doublet which coincides with the first diaphragm 16.
• the first diaphragm 16 therefore allows, through its opening, for example to control the degree of spatial inconsistency of the source 5 and/or the quantity of light received by the sample and/or the numerical aperture of illumination of the set 1 ... Furthermore, the first diaphragm 16 is also arranged in a focal plane of the second optics 15 and preferably in the focal plane obj and of the second optics 15.
• the focal length of the second optic 15 must be less than or equal to the distance separating the first optic 14 from the first diaphragm 16.
• diaphragm we mean for this description any organ making it possible to control the passage of the ray- light generated by the source 5 iris diaphragm, hole in a dedicated wall ...
• the interference device 4 comprises a second diaphragm 17 arranged downstream of the first adjustment unit 11 between the first adjustment unit 11 and the separator element 10.
• the second diaphragm 17 is arranged downstream of the second optic 15 between the second optic 15 and the separator element 10.
• the second diaphragm 17 is a field diaphragm.
• the second diaphragm 17 makes it possible to restrict the illumination of the sample to illuminate only the portion of the sample which will be imaged by assembly 1 and/or to reduce incoherent reflections.
• upstream of the separator element 10 is thus successively the source 5, the first optic 14, the first diaphragm 16, the first adjustment unit 11, the second optic 15 and the second diaphragm 17.
• the first optics 14, the first diaphragm 16, the second optics 15 and the second diaphragm 17 are fixed in module 3.
• the second optic 15 and the second diaphragm 17 are carried by the base.
• the second optic 15 and the second diaphragm 17 are arranged in the extension of the separator element 10.
• the source 5, the first optics 14 and the first diaphragm 16 are carried by the same portion of the frame and offset from the base.
• the source 5 therefore illuminates the separator element 10, which makes it possible to define a “lighting arm” of said separator element 10. Furthermore, it is known that the separator element 10 makes it possible to form two arms following its illumination by the source:
• an arm called an “object arm” which is associated, in operation, with the sample.
• the interference device 4 also includes a second adjustment unit 18 via which the reflection surface 6 will be able to interact with rays propagating from the separator element 10 on the reference arm.
• the second adjustable unit 18 comprises at least one reflection surface 27.
• the second adjustment unit 18 is arranged so that in use, a ray coming from the separator element 10 is reflected on the surface of reflection 27 to reach the reflection surface 6.
• the reflection surface 27 is flat.
• the reflection surface 27 is for example a mirror.
• said reflection surface 27 is mounted movable with respect to the frame of module 3.
• the reflection surface 27 can pivot relative to the frame.
• the second adjustment unit 18 comprises a kinematic mount carrying the reflection surface 27 (and allowing said reflection surface 27 to be moved with respect to the frame).
• the reflection surface 6 is itself movably mounted in the interference device 4 relative to the frame in order to be able to be moved relative to the sample during the study thereof.
• the reflection surface 6 is mounted on a base which can be moved in translation with respect to the frame.
• the base can be moved in translation with respect to the frame via at least one piezoelectric actuator.
• the base can be moved in a translational movement parallel to but not coincident with the optical axis of source 5.
• the interference device 4 here comprises a third optic 19 arranged between the separator element 10 and the reflection surface 6.
• the third optic 19 is for example a lens, a doublet...
• the third optic 19 is for example a doublet achromatic lens comprising an achromatic converging lens and preferably an achromatic converging lens having a flat face which is that facing the separator element 10.
• the third optic 19 makes it possible, for example, to facilitate balancing between the object arm and the reference arm and/or to correctly illuminate (ie over a large field) the reflection surface 27.
• the assembly 1 comprises a first objective 20 and a second objective 21.
• the two objectives 20, 21 are identical and are associated respectively with the one of the arms.
• the two lenses have an identical numerical aperture (better known by the acronym NA).
• NA numerical aperture
• the numerical aperture of the objectives is high. By “high” we mean a numerical aperture greater than 0.8 and preferably greater than 1 for the present application.
• the second optics 15 makes it possible to image the source 5 on a focal plane of the two objectives and for example on the object focal plane of the two objectives 20, 21.
• the first objective 20 is part of the module 3 and here of the interference device 4. Thus the first objective 20 is arranged in the module 3 at the level of the reflection surface 6.
• the optical axis of the first objective 20 is for example normal to a plane along which the reflection surface 6 extends.
• the first objective 20 is arranged so that the reflection surface 6 is in one of the foci of the first objective and for example at the image focal point of the first objective 20.
• the first objective 20 is therefore on the reference arm.
• the second adjustment unit 18 also comprises a member 26 for moving the first objective 20 relative to the frame and in particular relative to the reflection surface 6.
• the first objective 20 is carried by a base which is moved via the movement member.
• the movement member is configured to be able to move the first objective 20 along at least two axes of translation.
• the movement member is configured to be able to move the first objective 20 at least in a plane normal to the axis along which the reflection surface 6 can be moved with respect to the frame.
• downstream of the separator element 10, on the reference arm side there is thus successively the third optic 19, the second adjustment unit 18, the first objective 20 (associated with the organ displacement 26) and the reflection surface 6.
• the second objective 21 is not part of module 3. In reality the second objective 21 is directly the objective (or one of the objectives) of the microscope 2.
• the sample is intended to be positioned at one of the focal points of the second objective 21 and for example at the image focal point of the second objective 21.
• the second objective 21 is on the object arm when the microscope 2 and the module 3 are coupled.
• the second objective 21 is that of the microscope, module 3 alone cannot be sufficient to form a complete interferometer.
• the second objective 21 is arranged so as to observe the sample from below the sample.
• the second objective 21 is arranged under the plate and in this case under the incubator 9.
• the microscope 2 comprises a reflection surface 22 so that a ray passing through the second objective 21 along the optical axis of said second objective 21 can be reflected as far as the optical output of the microscope 2.
• the reflection surface 22 is planar.
• the reflection surface 22 is a mirror and for example a thick mirror and for example a mirror present- both a thickness greater than or equal to 3 millimeters and for example a thickness greater than or equal to 4 millimeters.
• said reflection surface 22 is a plane mirror carried by a prism or a plane mirror carried by a cube.
• said reflection surface 22 is arranged so that a ray propagating along the optical axis of the second objective 21 is then propagated, after reflection on the reflection surface 22, to exit via the optical output of the microscope 2.
• the module 3 is connected to the microscope 2, such a ray thus propagates from said output to the separator element 10 along the object arm.
• the interference device 4 further comprises a fourth optic 23 arranged between the separator element 10 and an “object arm” output of the module, ie the output of the module coupled at least optically with the optical output of the microscope 2.
• the fourth optic 23 is for example a lens, a doublet...
• the fourth optic 23 is for example an achromatic doublet comprising an achromatic converging lens and preferably an achromatic converging lens having a flat face which is that facing the separator element 10.
• the fourth optic 23 is associated with at least one member for moving the fourth optic 23 relative to the frame and in particular with respect to the separator element 10 (in particular to approach or move back the fourth optic 23 of the element separator 10).
• the fourth optic 23 is carried by a base which is moved via the displacement member.
• the movement member is configured to move cer the fourth optic 23 according to at least one translation.
• the displacement member is configured to move the fourth optic 23 according to at least one translation along the working axis of the module (ie the axis along which the majority of the light rays propagating on the object arm exit the module to reach the microscope).
• the fourth optic 23 is arranged in the module so as to be placed as close as possible to the reflection surface 22.
• the fourth optic 23 is arranged so that the distance between the second objective 21 and the fourth optic 23 is equal to the focal length of said fourth optic 23.
• the third optic 19 is arranged so that a focal plane of the third optic 19 coincides with a focal plane of the first objective 20, for example that the image focal plane of the third optic 19 coincides with the object focal plane of the first objective 20.
• the fourth optics 23 is arranged so that a focal plane of the fourth optics 23 coincides with a focal plane of the second objective 21, for example that the image focal plane of the fourth optics 23 coincides with the object focal plane of the second objective 21.
• the second diaphragm 17 is arranged in a focal plane of the fourth optic 23 via the separator element 10, and by example in the object focal plane of the fourth optic 23.
• the second diaphragm 17 is conjugated to the sample via the second objective 21 (the sample being at a focus of the second objective 21 and for example at the image focus of the second objective).
• the second diaphragm 17 is arranged in a focal plane of the third optic 19 via the separator element 10, and for example in the object focal plane of the third optic 19.
• the third optic 19 and the fourth optic 23 must be arranged in an identical manner with respect to the separator element 10.
• the module 3 comprises a fifth optic 24 arranged at the output of the interference device 4, that is to say arranged between the separator element 10 and the acquisition device 7.
• the fifth optic 24 can be part of the interference device 4 or may not be part of said interference device 4.
• the fifth optic 24 is a single lens, a single doublet or a pair of lenses or a pair of doublets. If the fifth optic 24 is a pair of doublets, the fifth optic 24 is composed for example of a first achromatic doublet (i.e. a set of an achromatic converging lens and a plane lens corrected to infinity upstream) and a second achromatic doublet (i.e. a set of an achromatic converging lens and a plane lens corrected to infinity downstream), the second doublet being arranged downstream of the first doublet.
• Flat faces lenses are respectively turned towards the acquisition device 7 and the separator element 10.
• the fifth optic 24 is arranged to combine the planes located at the foci of the two objectives 20, 21 (for example the planes located at the image foci of the two objectives 20, 21) in the same plane at the output of the interference device 4.
• the optical sensor of the acquisition device 7 is placed in this last plane. The optical sensor is thus arranged in a focal plane of the fifth optic 24 and for example in the image focal plane of the fifth optic 24.
• a focal plane of the fourth optics 23 is conjugated to a focal plane of the fifth optics 24 and for example an image focal plane of the fourth optics 23 is conjugated to the object focal plane of the fifth optics 24.
• the interference device 4 comprises a third diaphragm 25 arranged upstream of the fifth optic 24, between the fifth optic 24 and the separator element 10.
• the third diaphragm 25 is a field diaphragm.
• This third diaphragm makes it possible to adjust the optical position of the optical sensor and for example to reduce incoherent reflections.
• the second diaphragm 17 is thus arranged so as to be conjugated to the third optic 19 and to the fourth optic 23 and to the fifth optic 24 via the separator element 10.
• the third diaphragm 25 is arranged in a focal plane of the third optic 19 via the separator element 10, and by example in an image focal plane of the third optic 19.
• the third diaphragm 25 is conjugated to the reflection surface 6 via the first objective 20 (the reflection surface 6 being at one of the foci of the first objective 20 and by example in focus image of the first objective 20).
• the third diaphragm 25 is arranged in a focal plane of the fourth optic 23 via the separator element 10.
• the third diaphragm 25 is arranged in the image focal plane of the fourth optic 23 by the intermediate of the separator element 10.
• the third diaphragm 25 and the optical sensor are also combined (via the fifth optic 24).
• the focal length(s) of the first optics 14 are thus chosen as a function of the divergent character of the source 5, the distance between the source 5 and each of the objectives 20, 21 and the dimension of a pupil of a user to the focal planes objects of the objectives 20, 21.
• the first diaphragm 16 is conjugated, via the second optics 15 and the third optics 19/fourth optics couple 23, to the focal planes of the objectives 20, 21 and for example to the object focal planes of the objectives 20 , 21.
• the fourth optics 23 makes it possible to image the second diaphragm 17 on the sample.
• the second diaphragm 17 is placed at the focal distance of the second optic 15.
• the relative positioning of the second objective 21 on the one hand with respect to the source 5 and the reflection surface 6 on the other hand is essential.
• the microscope 2 is coupled to the module 3, the optical axis of the second objective 21 is in fact in a fixed position with respect to the working axis of the module 3.
• the two adjustment units 11, 18 make it possible to correctly position the source 5 and the reflection surface 6 with respect to the second objective 21, in particular to allow the generation of interference between the reference waves and the waves ob j and.
• reflection surface 27 is configured to (thanks to its relative movement with respect to the frame) align the separator element group 10/third optics 19/reflection surface 18/first objective 20 with the separator element group/fourth optics 23/reflection surface 22/second objective.
• Module 3 is thus easily inserted into microscope 2 and then the characteristics of module 3 are adjusted via the two adjustment units 11, 18 to optically align module 3 and microscope 2.
• the adjustment unit 18 comprising in particular the displacement member 26
• the adjustment unit 11 to modify the lighting arm if necessary in order to align the working axis of module 3 with the propagation axis of the source 5.
• module 3 can be connected to various microscopes on the market.
• the assembly 1 thus described is an improvement of a Linnik interferometer in a Koehler illumination configuration.
• the separator element 10 is much further away from the two objectives 20, 21 than in the systems of the prior art.
• This advantageously allows module 3 to be coupled to a conventional microscope.
• This also makes it possible to use objectives (the first objective 20 like the second objective 21) having a greater numerical aperture.
• the presence of at least one optic downstream of the separator element 10, on the object arm side makes it possible to improve the quality of the images resulting from the signals generated in the assembly 1.
• the incoherent reflections are reduced by the third diaphragm 25 then spatially confined to the center of an acquisition surface of the optical sensor (when said acquisition surface is centered with respect to an axis normal to a separation surface of the separator element) ) . It therefore proves easier for the processing device 8 to separate said incoherent reflections from coherent reflections and thus to obtain a better quality image.
• the processing device 8 is here configured to synchronize the acquisition device 7 (and in particular its optical sensor) with the actuator allowing the movement of the reflection surface 6.
• the processing device 8 can also include an acquisition card connected to the computer to ensure this synchronization.
• the cells can for example be two-dimensional cultures such as monolayer two-dimensional cultures, three-dimensional cultures such as organoids or many other multilayer three-dimensional cultures...
• the set 1 described can be used for example for the study of organoids, two-dimensional single-layer cultures, three-dimensional multilayer cultures, retinas and corneas, the study of explants of retinas and corneas of mice, pigs, macaques, etc., quality control of the production of organoids on a large scale, helping in the micro-fluidic field, the field of optogenetics (for example by photo-stimulation for 1 'optophysiology), disease modeling, to carry out effectiveness tests of new treatments (genetic, pharmaceutical, etc.), for transplantation, etc.
• the assembly 1 described makes it possible to generate a static signal making it possible to visualize the three-dimensional structure of a tissue as well as a dynamic signal making it possible to identify the cells of a tissue and to measure them by example their metabolism.
• microscopy studies with high spatial resolution (for example a resolution of between 100 and 400 nanometers) and/or temporal resolution (for example a resolution of the order of millisecond such as for example 2 milliseconds) in particular those excluding the destruction of the sample and/or integrating the absence of endogenous markers.
• high spatial resolution for example a resolution of between 100 and 400 nanometers
• temporal resolution for example a resolution of the order of millisecond such as for example 2 milliseconds
• the incubator may or may not be part of the assembly and/or the acquisition device may or may not be part of the assembly and/or the processing device may or may not be part of the assembly and/or or the source may or may not be part of the whole.
• the acquisition device may or may not be part of the module and/or the processing device may or may not be part of the module and/or the source may or may not be part of the module. be part of the module or not.
• the module may include one or more glass blades to limit dispersion phenomena.
• the microscope used is not provided with a flat reflection surface between its objective and an optical output
• the microscope can of course be equipped with such a flat surface.
• a flat reflection surface in the module between the fourth optics and the working output of the module or else arrange such a flat surface in another module itself inserted in one of the rows of the microscope to be associated to the invention.
• the module is coupled to the microscope by simple insertion of the module into the microscope, in addition or as a replacement, the module and the microscope can be coupled together by cooperation, one of a male connector and the other of a female connector, the two connectors being able to cooperate together for the connection of the module to the microscope.
• the module may include a male connector and the microscope a female connector.
• the module includes a threaded rod capable of being screwed into a corresponding threaded orifice of the microscope.
• the microscope in the assembly could be a microscope without a turret.
• the microscope in the set may not be an inverted microscope.
• the illumination of the sample can thus be carried out from above (the collection of the signal by the second objective then taking place preferentially from above as well) as well as from the bottom (the collection of the signal by the second objective taking place then preferably from the bottom as well).
• the third optic can be included in the microscope and not in the module.
• the optical sensor may be different from what has been indicated, for example the optical sensor may be a charge-coupled sensor (better known by the English term CCD for Charge-Coupled Device).
• the optical sensor may be able to work in the visible and/or in another domain such as for example in the infrared.
• the optical sensor could be a near infrared image sensor (better known by the English term SWIR sensor for Short-Wave-Inf rare).
• the optical sensor could for example be an InGaAs sensor (for indium-gallium arsenide) or even an InGaAs SWIR sensor.
• the module and/or the assembly may be shaped so that the optical sensor (and/or the acquisition device) is interchangeable in order, for example, to be able to work in the visible and then to be able to work in a domain other than the visible. and for example in the infrared.
• the set may not include an incubator (portable or not).
• the assembly may include a heating enclosure in which the microscope is at least arranged to be able, for example, to maintain the sample at a given temperature.
• the optics all have lenses with at least one flat face, the lenses could be shaped differently.
• the lenses may also be oriented differently than indicated.
• a lens will be arranged in the module of so that the light beam having a largest opening angle (between the incoming or outgoing luminant beam) is associated with the face of the flattest lens.

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• 2022
  • 2022-04-22 WO PCT/FR2022/000042 patent/WO2023203283A1/fr not_active Ceased
  • 2022-04-22 EP EP22725520.5A patent/EP4511610A1/fr active Pending
  • 2022-04-22 JP JP2024562898A patent/JP2025513579A/ja active Pending
  • 2022-04-22 US US18/858,589 patent/US20250277965A1/en active Pending
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