Patent Application
20230298855
The invention relates to a method and an apparatus for micromachining a sample using Focused Ion Beam, and a correlative inspection apparatus for performing said method. In particular, the invention relates to an apparatus and method for micromachining samples by means of a focused ion beam, to produce samples suitable for inspection in a charged particle beam inspection apparatus, for example an electron microscope.
Focused Ion Beam (FIB) micromachining for Electron Microscopy (EM) samples is a preparation method which allows to machine samples with high precision and without inducing mechanical artefacts, as for example induced by ultra-microtomy. In addition, dual beam systems combining a FIB with a Scanning Electron Microscope (SEM) are known in the art. These dual beam systems allow to use the SEM to image the sample for navigating and positioning the sample in order to machine a position of interest, and for parallel monitoring of the micromachining process by the FIB.
An example of such a system is described in U2020/0027692 A1. It is noted that this document describes a dual beam system combining a FIB and a SEM, and a separate optical microscope or SEM may be used to study the surface of the sample prior to mounting the sample in the dual beam system.
It is noted, that the micromachining of a sample by means of a FIB can be used, for example, for the manufacturing of lamella (thin slices) of the sample, which are typically imaged using a Transmission Electron Microscope (TEM).
However, when using such a SEM/FIB system for micromachining beam-sensitive samples, such as for example organic material, the sample may be altered and artifacts may be induced by the electron beam of the SEM, which is undesirable, particularly in those cases where the sample is being processed for high resolution inspection in a Transmission Electron Microscope.
For example, the presence of free charge carriers (electrons or possibly holes) may make the sample vulnerable to chemical reactions, such as decomposition due to bond breakage or reactions involving radical or ionized intermediates. Similarly, also the excitation of bound electrons to high energy, weakly bound states as a result of the cascade of energy dissipation reactions after electron beam irradiation, can lead to chemical modification.
Especially organic materials, such as biological material, polymers, and other soft matter, are for this reason hard to image by means of an electron microscope. However, also inorganic materials may be prone to electron-irradiation induced damage. And even for conducting materials, the decomposition of absorbed gas molecules present in the electron microscope vacuum chamber can modify the surface structure such that the imaging quality is negatively affected.
It is an object of the present invention to provide a method for micromachining vulnerable and/or dynamic materials using a FIB, and preferably to provide lamella from a position of interest of the sample in a substantially undamaged state or in a way that minimizes the chance for imaging artefacts or sample modification by non-invasive determination of regions of interest in-situ in an assembly comprising a FIB apparatus.
In addition or alternatively, it is an object of the present invention to provide a method to monitor the sample during micromachining of the sample by means of a FIB.
According to a first aspect, the present invention provides a method for micromachining a sample using an apparatus for micromachining samples, wherein the apparatus comprises an integral combination of:
The method of the present invention uses an apparatus in which a Focused Ion Beam (FIB) exposure system and a light optical microscope (LM) are integrated, such that a light beam and/or the FIB can interact subsequently and/or simultaneous with a sample on the sample holder. Preferably, the apparatus only comprises the FIB exposure system and the LM. Since the FIB exposure system and the LM are part of an integral combination, their alignment with respect to each other is at least partially based on the design of the apparatus, and if necessary, can be fine-tuned using for example a marker that can be produced or activated by the FIB and that can be identified by the LM. Accordingly, the relative orientation of the FIB and the LM is or can be established and allows to provide a geometric translation between the LM and the FIB exposure system.
The present invention is based on the realization that such an integral system allows for highly accurate determination of regions of interest in the specimen in a non-invasive manner by using the light optical microscope. The integrated LM/FIB apparatus can thus be used to locate an area within the sample where there is a region of interest using only the light optical microscope.
In addition, due to the known spatial relation between the FIB and the LM, the integrated LM/FIB apparatus of the present invention can establish from the one or more light microscopy images or measurements, how and where the FIB can be employed for micromachining the sample to remove material from the surface of the sample in order to reduce a distance between at least part of the region of interest and the surface of the sample or to produce a lamella which embodies at least part of the region of interest, in particular to allow the region of interest to be studied later by an electron microscope. In particular, the apparatus for micromachining of samples is configured to establish from the one or more LM images, one or more settings of the sample holder and/or the FIB exposure system. Such settings may include, but are not limited to: the dimensions of the focus of FIB, the beam current of the FIB, and position coordinates for the sample holder for positioning the sample in order to allow the FIB to be applied at a desired and/or predetermined position on the sample.
In case the current position of the sample does not allow to apply the FIB at the desired and/or predetermined position on the sample, the sample holder can be used to orient and/or position the sample with respect to the FIB such that the first position is arranged on the sample relative to the at least part of the region of interest for the micro-machining of the sample using the FIB. In addition, or alternatively, the trajectory or intended trajectory of the FIB can be adjusted or arranged to the first position on a desired position on the sample. It is noted that the FIB system preferably comprises deflectors for adjusting the trajectory of the FIB. The settings of these deflectors can be set in order to adjust the intended trajectory of the FIB, prior to activating the FIB.
Subsequently, the FIB can be activated to start the micromachining process of the sample.
According to the method of the invention, the determination of the location of a region of interest and navigating and positioning of the sample for machining the sample using the FIB is performed using the light optical microscope that is integrated with the FIB exposure system. The method of the invention allows to identify the location of a region of interest and to navigate and position the sample in the integrated LM/FIB apparatus of the present invention without a prior charged particle beam exposure of said region of interest. Also, during the micromachining of the sample by the FIB, no prior electron beam exposure of said region of interest is required. The present invention thus provides a method for micromachining vulnerable and/or dynamic materials using a FIB, and to remove material from the sample in order to make the layer of material between the surface of the sample and the region of interest at least thin enough to be able to study the region of interest by means of a transmission electron microscope. Preferably, the method of the present invention is configured to expose at least part of the region of interest of the sample at the surface. Accordingly, the method of the invention allows micromachining the sample such that the region of interest remains in a substantially undamaged state or in a way that minimizes the chance for introducing imaging artefacts or sample modifications. By micromachining the sample to reduce the distance between the region of interest of the sample and the surface of the sample, this part of the region of interest is readily available to be studied by an electron microscope.
In an embodiment, the method further comprising the step of: establish from the one or more light microscopy images which part or parts of the sample need to be micro-machined by the focused ion beam exposure system to bring at least part of the region of interest more closely to the surface of the sample or to produce a lamella which embodies at least part of the region of interest. Preferably, the method is configured to establish from the position and physical dimensions of the region of interest as determined using the light optical microscope, and preferably from this information alone, which part or parts of the sample need to be removed by the FIB to reduce a distance between at least part of the region of interest and the surface of the sample or to produce a lamella which embodies at least part of the region of interest. In addition, the method may also be configured to establish the best way the sample should be machined without substantially damaging the region of interest and/or without substantially introducing artefacts and/or modifying the surface structure of the sample.
In an embodiment, the settings comprise a to be machined position on the sample where to arrange the first position, wherein the method further comprises the step of: moving the sample or at least an intended trajectory of the focused ion beam to locate the first position on the to be machined position on the sample accordingly, preferably before activating the focused ion beam exposure system for micromachining the sample. Preferably, the method is configured to provide a geometric translation between the information from the sample as obtained by the light optical microscope which information provides a to be machined position on the sample, and a positioning of the sample by the sample holder with respect to the trajectory of the FIB, such that the FIB, in use, directly impinges on the sample at the to be machined position. Accordingly, the method allows to maneuver the sample in such a way that the sample or a part thereof does substantially not interfere with the trajectory of the FIB.
In an embodiment, the method further comprises the step of: monitoring the locating of the first position on the sample and/or monitoring the micromachining of the sample using the light optical microscope. The light optical microscope according to this embodiment is configured for imaging or monitoring said first position. The method of the present invention allows to ascertain that the sample is properly positioned so that in use the FIB impinges on the to be machined position, and/or to monitor the sample during micromachining of the sample by means of a FIB.
In an embodiment, the method comprises the step of setting the spot size and/or the beam current of the FIB based on the one or more light microscopy measurements. By setting the spot size and/or the beam current of the FIB, the area and volume of material that is machined by the FIB can be selected. Based on the information obtained by the light microscopy measurements, the spot size and/or the beam current can be set to a relatively large value when a distance between the surface of the sample and the region of interest is large and a large amount of sample material has to be removed to at least reduce the distance between the region of interest and the surface. Alternatively, and again based on the information obtained by the light microscopy measurements, the spot size and/or the beam current can be set to a relatively low value when the distance between the surface of the sample and the region of interest is small and a small amount of sample material has to be removed carefully to reduce the distance between the region of interest and the surface, or to expose the region of interest at the surface, preferably without damaging the region of interest.
In an embodiment, the light optical microscope comprises a super resolution microscopy system, including types that use structured illumination, wherein the super resolution microscopy system provides position information of at least part of the region of interest with a resolution of approximately 300 nm or smaller. This allows to more accurately determine the position and physical dimensions of the region of interest in the sample. The use of a super resolution technique is particularly useful for micro-machining the sample for manufacturing one or more lamella suitable to be studied in a Transmission Electron Microscope (TEM). In order to allow an electron beam to at least partially be transmitted through a sample, this sample needs to be very thin, for example having a thickness of approximately 100 nm. The use of super resolution techniques allows the LM/FIB apparatus of the present invention to micro-machine such thin samples which include at least part of the region of interest.
It is noted that a light optical microscope is much more sensitive to deviation in a direction parallel to the optical axis of the light optical microscope than, for instance, an electron microscope. Accordingly, the light optical microscope can be used to determine the position of the sample and/or the region of interest in the sample, at least in a direction parallel to the optical axis with high precision, even if the light optical microscope is not a super resolution microscopy system.
In an embodiment, the light optical microscope comprises a fluorescence light optical microscope, wherein the method further comprises the step of providing structures around the region of interest with first fluorescent labels which can be observed by the light optical microscope. Preferably, the micromachining is monitored by using fluorescence light from said first fluorescent labels. As such, when the fluorescence of the first fluorescent labels as detected with the light optical microscope goes down in intensity, this is a sign that the FIB is approaching the region of interest. Accordingly, micromachining of the sample can be accurately controlled by monitoring changes in the fluorescence intensity of the first fluorescent labels.
In addition or alternatively, in an embodiment, the method comprises the step of providing the region of interest with second fluorescent labels which can be observed by the fluorescence light optical microscope. Preferably, the micromachining is monitored by using fluorescence light from said second fluorescent labels. As long as the fluorescence of the second fluorescent labels as detected with the light optical microscope does not at least substantially go down in intensity, this is a sign that the region of interest is still enclosed in the sample and/or lamella. Accordingly, micromachining of the sample can be accurately controlled by monitoring changes in the fluorescence intensity of the second fluorescent labels.
It is noted that when using both the first and the second fluorescent labels, the second fluorescent labels are preferably different from the first fluorescent labels, so that they are distinguishable in measurements in a fluorescence light microscope. For example, the fluorescence spectrum of the first fluorescent labels differs from the fluorescence spectrum of the second fluorescent labels, preferably in manner that is distinguishable by the fluorescence light optical microscope. Furthermore, the first and/or the second fluorescent labels may comprise a fluorescent protein. Fluorescent proteins are very suitable for labeling regions of interest in biological specimens or samples.
In an embodiment, the method of the invention comprises the step of manufacturing one or more lamella from the sample which includes at least part of the region of interest. In this respect, a lamella is a thin cut-out from a thicker sample, preferably with a thickness suitable for studying the lamella in a TEM. Such a lamella includes the at least part of the region of interest which can later be studied in a TEM. Subsequently, the sample holder and/or the (intended) trajectory of the FIB can be oriented and/or positioned with respect to each other such that the first position is arranged on the sample for the manufacturing of the lamella which includes at least part of the region of interest. Subsequently, the FIB can be activated to start the micromachining process for making the lamella.
In an embodiment, the to be produced lamella is configured to comprise an observation surface, wherein the apparatus for micromachining the sample is configured to orient the sample and the FIB with respect to each other such that the FIB impinges on the sample at an oblique or grazing angle with respect to said observation surface. As indicated above, the lamella with the at least part of the region of interest are intended to be studied in an TEM. Accordingly, the lamella is a very thin section of the sample which is configured to be studied in an electron microscope in transmission. When studied in the electron microscope, the electron beam passes at least partially through an upper and lower surface of the lamella, and the transmitted electron beam is used to provide a transmission image of the lamella. The surfaces through which the electron beam passes are referred to herein as observation surfaces. By arranging the sample and the FIB with respect to each other such that the FIB impinges on the sample at an oblique or grazing angle with respect to said observation surface, it can at least substantially be prevented that ions from the FIB are implanted in the lamella surface. Accordingly, the method according to this embodiment further reduces the chance that the lamella that is provided comprises artefacts due to the micromachining of the sample using the FIB.
In an embodiment, the method further comprises the step of monitoring the creation of the lamella using the light optical microscope, preferably using a super resolution technique, such as the above described fluorescent labeling of the sample. Accordingly, the same light optical microscope that is used to identify the region of interest, is also used to monitor the creation of the lamella. In an embodiment, the method further comprises the step of determining how close the lamella is to containing at least a part of the region of interest and/or determining an angle of approach between the FIB and the region of interest. In an embodiment, the monitoring step of the previous embodiment(s) is used to determine whether at least a part of the region of interest is still enclosed within the lamella. Accordingly, these embodiments of the method of the present invention allow to control the micro-machining in order to obtain a lamella with at least a part of the region of interest.
In an embodiment, the monitoring step of the previous embodiment(s) is used to determine and/or correct a drift of the sample position, at least during the creation of a lamella, in particular at least a drift in a direction parallel to an optical axis of an objective lens of the light optical microscope. In particular when using a high resolution optical objective lens and/or a confocal light microscope arrangement, the light optical microscope is very sensitive to deviations in a direction parallel to the optical axis of the objective lens. Deviations of less than one micrometer can easily be determined. Accordingly, this allows for easy tracking of the focus position.
In an embodiment, the method further comprises the steps of:
Preferably, the lamella is evaluated in a separate TEM, which thus is not integral with the integral FIB/LM apparatus of the present invention. From the TEM or cryo-TEM measurements it can be established whether or not the lamella as produced by the FIB actually contained at least part of the region of interest and/or a protein of interest. Based on the data from the TEM or cryo-TEM the method for manufacturing the lamella in the integrated LM/FIB apparatus can be improved to increase the probability that a next lamella manufactured with this apparatus indeed comprises the desired part of the region of interest and/or the protein of interest.
In an embodiment, the sample holder comprises a cooling system for cooling the sample, wherein the method further comprises the step of cooling the sample prior to the micromachining of the sample by the FIB, preferably cooling the sample down to a cryogenic temperature. In particular for organic or other vulnerable samples which are commonly studied in a cryo-TEM it is advantageous to perform the micromachining on a cooled sample, preferably on a sample which is already cooled down to a cryogenic temperature so that the sample after being micro-machined by the FIB is readily available for investigation in a cryo-TEM.
In an embodiment, the sample is cooled prior to a positioning of the sample in the sample holder. Accordingly, the sample holder does not need to cool the whole sample but only needs to maintain the low temperature of the sample, and the cooling capacity of the cooling system of the sample holder does not need to be very high such that a relatively small cooling system may be sufficient in this case.
In an embodiment, the light optical microscope comprises a focus tracker, wherein the method further comprises the step of focusing the light optical microscope on the sample holder, and/or focusing the light optical microscope on a lamella that is being created by micromachining the sample using the focused ion beam exposure system.
According to a second aspect, the present invention provides an apparatus for micromachining a sample, wherein the apparatus comprises an integral combination of:
Preferably the apparatus further comprises a controller which is configured for controlling the apparatus to perform, in use, the steps of the method or an embodiment thereof as described above.
The apparatus of the invention is configured to use the light optical microscope to determine the location of a region of interest and navigating and/or positioning of the sample prior to machining the sample using the focused ion beam (FIB) exposure system. In particular due to the integral combination of the light optical microscope and the FIB exposure system, the apparatus of the invention allows to identify the location of a region of interest and to navigate and position the sample in the integrated LM/FIB apparatus of the present invention without a prior charged particle beam exposure of said region of interest. Preferably, said apparatus is configured for performing the method as described above, or an embodiment thereof.
In an embodiment, the light optical microscope comprises a cylindrical lens, wherein the cylindrical lens is preferably arranged in a light optical path towards a detector of the light optical microscope. In an embodiment, the cylindrical lens is a first cylindrical lens, wherein the light optical microscope comprises a second cylindrical lens which is preferably arranged adjacent to the first cylindrical lens, and wherein a cylinder axis of the second cylindrical lens is arranged at an angle θ with respect to the cylinder axis of the first cylindrical lens, wherein the angle θ is defined in a plane perpendicular to the optical axis of the light optical path towards the detector. Preferably the angle θ is larger than 0 degrees and smaller than 360 degrees. By providing the light optical microscope with a cylindrical lens, In particular in the light optical path towards the detector of the light optical microscope, the resolution in a direction along an optical axis of an objective lens of the light optical microscope can be improved.
In an embodiment, the light optical microscope comprises an optical objective lens having an optical axis, wherein the apparatus comprises a mirror which is arranged on the optical axis at a position spaced apart from the optical objective lens, and wherein the sample holder is configured for holding a sample in between the optical objective lens and the mirror. Preferably, said mirror comprises a flat mirror. By providing the apparatus with a mirror in the orientation as defined above, the resolution in a direction along an optical axis of an objective lens of the light optical microscope can be improved.
In an embodiment, the light optical microscope comprises a focus tracker. Preferably the focus tracker is configured to focus the light optical microscope on the sample holder, and/or on a lamella that is being created by micromachining the sample using the focused ion beam exposure system. In use, the focus tracker keeps the sample in the focus of the light optical microscope. In addition or alternatively, the focus tracker provides information about the position of the sample in a direction along the optical axis of the light optical microscope. This information can be used to control the positioning of the sample by the sample holder before and/or during applying the FIB for micro-machining the sample.
In an embodiment, the light optical microscope is a fluorescence microscope and/or a super resolution light optical microscope. By incorporating a fluorescence microscope and/or a super resolution light optical microscope the resolution of the LM can be improved as described in more detail above.
In an embodiment, the sample holder comprises a cooling system for cooling the sample, preferably wherein the cooling system is configured for cooling the sample down to a cryogenic temperature. This allows to micro-machine the sample under cryogenic conditions.
In an embodiment, the apparatus further comprises:
Accordingly, the apparatus for micromachining of samples comprising an integral combination of a sample, a focused ion beam exposure system, and a light optical microscope, is further provided with an integral arranged TEM. This TEM allows evaluation of the micro-machined sample, in particular the lamella as produced with the FIB. The result of said evaluation can be used to provide feedback to the apparatus for micromachining a sample to improve the targeting of a region of interest in a subsequent micromachining of a lamella.
In an embodiment, the detector system comprises a sheet of a scintillator material, wherein the sheet of scintillator material is arranged in between a position on the sample holder where, in use, a sample is positioned, and an objective lens of the light optical microscope, wherein the light optical microscope is configured for acquiring an image of at least a part of the sheet of the scintillator material. In an embodiment, the apparatus comprises an actuator for moving the sheet of scintillator material from a first position where the scintillator material is arranged in between the position on the sample holder where, in use, a sample is positioned, and the objective lens of the light optical microscope, to a second position where the scintillator material is removed from the area in between the position on the sample holder where, in use, a sample is positioned, and the objective lens of the light optical microscope, or vice versa.
The various aspects and features described and shown in the specification can be applied, individually, wherever possible. These individual aspects, in particular the aspects and features described in the attached dependent claims, can be made subject of divisional patent applications.
The invention will be elucidated on the basis of an exemplary embodiment shown in the attached drawings, in which:
The light optical microscope comprises an objective lens 4, a light source 5 and a detector 9. The light source 5 is configured to direct light 7 from the light source 5 towards the objective lens 4, which is configured to focus the light onto the sample 20 on the sample holder 2. In the beam path in between the light source 5 and the objective lens 4, a half transparent mirror or dichroic mirror 6 is arranged, which is configured to pass at least part of the light 7 from the light source 5 towards the objective lens 4 to illuminate the sample 20.
The objective lens 4 is furthermore configured to collect light coming from the sample 20. The light collected by the objective lens 4 is at least partially reflected by the half transparent mirror or dichroic mirror 6 to direct said collected light 8 towards the detector 9.
Accordingly, the light optical microscope is configured to observe the sample 20 on the sample holder 2, taking optical measurement and/or optical images from the sample 20.
As schematically shown in
The focused ion beam exposure system 3 is typically arranged inside a vacuum chamber 11 which is connected to a vacuum pump via a connector 12.
As schematically shown in
Because of the integral combination of the light optical microscope and the focused ion beam exposure system 3, the optical axis OA of the light optical microscope and the focused ion beam 30 axis are at least partially linked by design. This relation between the optical axis OA of the light optical microscope and the focused ion beam 30 allows to establish from the one or more light microscopy measurements or images where (position) and how (spatial orientation) to position the sample 20 in order to machine the desired part(s) of the sample 20 with the Focused ion beam 30.
It is noted that the focused ion beam exposure system 3 is configured for projecting the focused ion beam 30 onto a first position 31. The sample 20 is positioned by the sample holder 2 so that the first position 31 at least substantially coincides with a position on the sample 20 which needs to be treated by the focused ion beam 30. Preferably, the first position 31 is arranged so that it can be imaged or monitored by the light optical microscope. In the example as shown in
It is noted, that the apparatus 1 preferably comprises a controller (not shown) which is connected to the light optical microscope, at least the detector 9 thereof, the focused ion beam exposure system 3, and the sample holder 2. The controller is configured for controlling the apparatus 1 to perform, in use, the steps of the method or an embodiment thereof as described below.
In use, light 7 from the light source 5 is directed towards the objective lens 4, which is configured to illuminate the sample 20. Light 8 from the sample is collected by the objective lens 4 and directed to the detector 9. In particular, the objective lens 4 is furthermore configured to collect light coming from the sample 20. The light collected by the objective lens 4 is at least partially reflected by the half transparent mirror or dichroic mirror 6 to direct said collected light 8 towards the detector 9. Preferably, the light optical microscope is configured to project an image of the sample surface onto the detector 9, wherein the detector 9 comprises a camera, for example a CCD camera, in order to capturing one or more light microscopy images of the sample 20 held by the sample holder 2.
Using the one or more light microscopy images as captured by the detector 9, a position and physical dimensions of a region of interest in the sample 20 can be determined. This determination can be performed by a user, for example by displaying said one or more light microscopy images on a display screen, wherein the user may select a part or a position in said one or more light microscopy images as a regions of interest. In addition or alternatively, this determination may be performed by a computing device or image analyzer, preferably using a predetermined contrast feature which enables the computing device or image analyzer to distinguish between the region of interest from the surrounding sample material.
Subsequently, the user and/or the computing device or image analyzer establishes from the one or more light microscopy images settings of the sample holder and/or the focused ion beam exposure system for micromachining the sample 20 to remove material form the surface of the sample 20 in order to reduce a distance between at least part of the region of interest and the surface of the sample 20 or to produce a lamella which embodies at least part of the region of interest, as will be explained in more detail below with reference to
Optionally, the light optical microscope is provided with a cylinder lens arrangement 10 arranged in the light optical path 8 towards the detector 9 of the light optical microscope, to improve the resolution of the light optical microscope along the optical axis OA. The cylinder lens arrangement 10 comprises a first cylindrical lens 101 and a second cylindrical lens 103 which is preferably arranged adjacent to the first cylindrical lens 101 in a direction parallel to the light optical path 8. The first cylindrical lens 101 comprises a cylinder axis 102 and the second cylindrical lens 103 comprises a cylinder axis 104. As schematically shown in the front view detail in
Optionally, the sample holder 2 is provided with a mirror 22 which is arranged on the optical axis OA at a position spaced apart from the optical objective lens 4, and wherein the sample holder 2 is configured for holding a sample 20 in between the optical objective lens 4 and the mirror 22. Preferably, said mirror 22 comprises a flat mirror. By providing the apparatus with a mirror 22 in the orientation as shown in
Again, the light optical microscope comprises an objective lens 104, a light source 105 and a detector 109, in a same configuration as in the first exemplary embodiment as described above with reference to
As schematically shown in
Optionally, the light optical microscope comprises a blocking filter 117 which is configured for at least substantially blocking the Infra-red light used by the focus tracker 115. The blocking filter 117 can at least substantially prevent that the Infra-red light used by the focus tracker 115, interferes with the light optical measurements by the light optical microscope.
As schematically shown in
The focused ion beam exposure system 103 is typically arranged inside a vacuum chamber 111 which is connected to a vacuum pump via a connector 112.
As schematically shown in
Because of the integral combination of the light optical microscope and the focused ion beam exposure system 103, the optical axis OA of the light optical microscope and the focused ion beam 130 axis are at least partially linked by design. This relation between the optical axis OA of the light optical microscope and the focused ion beam 130 allows to establish from the one or more light microscopy measurements or images where (position) and how (spatial orientation) to position the sample 120 in order to machine the desired part(s) of the sample 120 with the Focused ion beam 130.
Just as in the previous example, the focused ion beam exposure system 103 is configured for projecting the focused ion beam 130 onto a first position 131. The sample 120 is positioned by the sample holder 102 so that the first position 131 at least substantially coincides with a position on the sample 120 which needs to be treated by the focused ion beam 130. Preferably, the first position 131 is arranged so that it can be imaged or monitored by the light optical microscope. In the example as shown in
In use, light 107 from the light source 105 is directed towards the objective lens 104, which is configured to illuminate the sample 120. The objective lens 104 is furthermore configured to collect light coming from the sample 120. The light collected by the objective lens 104 is at least partially reflected by the half transparent mirror or dichroic mirror 106 to direct said collected light 108 towards the detector 109. In particular, the light optical microscope is configured to project an image of the sample surface onto the detector 109, wherein the detector 109 comprises a camera, for example a CCD camera, in order to capturing one or more light microscopy images of the sample 120 held by the sample holder 102. The focus tracker 115 can be used to position and hold the sample 120 on the sample holder 102 in focus, before or during the imaging.
Using the one or more light microscopy images as captured by the detector 109, a position and physical dimensions of a region of interest in the sample 120 can be determined. This determination can be performed by a user, for example by displaying said one or more light microscopy images on a display screen, wherein the user may select a part or a position in said one or more light microscopy images as a regions of interest. In addition or alternatively, this determination may be performed by a computing device or image analyzer, preferably using a predetermined contrast feature which enables the computing device or image analyzer to distinguish between the region of interest from the surrounding sample material.
Subsequently, the user and/or the computing device or image analyzer establishes from the one or more light microscopy images settings of the sample holder and/or the focused ion beam exposure system for micromachining the sample 120 to remove material form the surface of the sample 120 in order to reduce a distance between at least part of the region of interest and the surface of the sample 120 or to produce a lamella which embodies at least part of the region of interest, as will be explained in more detail below with reference to
From the one or more light microscopy images as obtained by the light optical microscope from the sample 20, the position of the region of interest 21 in the sample 20 can be established.
In addition, from the information from these light microscopy images, and preferably from this information alone, a preferred way to machine the sample 20 can be established in order to bring at least part of the region of interest 21 more closely to the surface of the sample 20 or to produce a lamella 22 which embodies at least part of the region of interest 21. In order to establish the preferred way to machine the sample 20, the apparatus of the present invention or a controller thereof is preferably configured to also take account of the topography of the surface(s) of the sample 20 and/or the relative orientation of the sample on the sample holder 2 with respect to the focused ion beam exposure system 3, in particular with respect to the focused ion beam 30 and/or the position of the focus of the focused ion beam 30, which focus is preferably arranged at or near said first position.
Furthermore, the apparatus of the invention or a controller thereof is preferably configured to arrange the sample 20 and the focused ion beam 30 with respect to each other such that the focused ion beam 30 impinges on the sample 20 at an oblique or grazing angle with respect to an intended observation surface 25, 25′, in order to at least substantially prevent that ions from the focused ion beam are implanted in said observation surface 25, 25′.
When the position of the region of interest 21 and a position and/or orientation of an intended observation surface 25 has been established, a preferred way to machine the sample 20 to remove the material 23 of the sample which is arranged at a side of the intended observation surface 25 facing away from the region of interest 21, is established as schematically shown in
Subsequently, the sample holder 2 is controlled to position the sample 20 with respect to the focused ion beam 30 such that the material 23 of the sample which is arranged at a side of the intended observation surface 25 facing away from the region of interest 21 can be removed as schematically shown in
The sample 20 as shown in
However, in order to study the region of interest 21 in great detail, the use of a Transmission Electron Microscope (TEM) is commonly preferred. In order to make the sample 20 suitable for studying the region of interest 21 with a TEM, the sample 20 must be further machined in order to obtain a lamella 22. Such a lamella uses the observation surface 25 as a first observation surface. In order to from a thin lamella 2, an intended second observation surface needs to be defined, which second observation surface is at least substantially parallel to the first observation surface, and preferably in such a way that at least part of the region of interest 21 is arranged in between the first and second observation surface. The intended second observation surface 25′ can be obtained by removing the material 23′ of the sample 20 which is arranged at a side of an intended second observation surface 25′ facing away from the region of interest 21, as schematically shown in
Accordingly, the sample holder 2 is controlled to position the sample 20 with respect to the focused ion beam 30 such that the material 23′ of the sample 20 which is arranged at a side of the intended second observation surface 25′ facing away from the region of interest 21 can be removed, preferably layer by layer 24′, as schematically shown in
It is noted, that instead of first machining the sample at the first side to expose the intended first observation surface and subsequently machining the sample at the second side to expose the intended second observation surface, the method of the present invention may also comprise the steps of:
The result of the micro-machining is a lamella 22 as schematically shown in
As schematically shown in
However, the sensitivity of observing a progress of the removal of material from the sample 40 can be increased by providing the material around the region of interest 41 with first fluorescent labels 46 which can be observed by the light optical microscope, as schematically shown in
In addition or alternatively, the region of interest 51 can be provided with second fluorescent labels 56 as schematically shown in
It is noted, that the interaction between the focused ion beam 30 and the sample material may result in an emission of secondary electrons. These secondary electrons may travel over tens of nanometers from the first position where the focused ion beam 30 impinges on the sample, which secondary electrons may then interact with any fluorescent labels 56 present, to induce changes in the fluorescence intensity. Accordingly, when using fluorescent labels 56 which interact with secondary electrons, a change in fluorescence intensity can be observed while the focused ion beam 30 is still tens of nanometers away from the region of interest 56, which may be used to further safeguard that the region of interest 56 is not machined by the focused ion beam 30.
It is further noted, that in case the sample is provided with both the first fluorescent labels 46 and the second fluorescent labels 56, it is preferable that the first fluorescent labels 46 are different from the second fluorescent labels 56, preferable such that the fluorescent light from the first fluorescent labels 46 has a different wavelength or wavelength range in comparison to the fluorescent light from the second fluorescent labels 56, and that the detector is configured to be able to distinguish between the fluorescent light from the first fluorescent labels 46 and the fluorescent light from the second fluorescent labels 56.
It is to be understood that the above description is included to illustrate the operation of the preferred embodiments and is not meant to limit the scope of the invention. From the above discussion, many variations will be apparent to one skilled in the art that would yet be encompassed by the scope of the present invention.
In summary, the invention relates to an apparatus and a method for micromachining samples. The apparatus comprises an integral combination of: a sample holder, a focused ion beam (FIB) exposure system for projecting a FIB onto a first position on the sample, and a light optical microscope (LM), wherein the LM is configured for imaging or monitoring said first position. The method comprises the steps of:
| Number | Date | Country | Kind |
|---|---|---|---|
| 2026054 | Jul 2020 | NL | national |
| Filing Document | Filing Date | Country | Kind |
|---|---|---|---|
| PCT/NL2021/050441 | 7/13/2021 | WO |
