How do Electron Microscopes Work? š¬š š¬ Taking Pictures of Atoms
Branch Education
0:00 Have you ever wondered how scientists and engineers design transistors
0:04 that are around the width of a strand of DNA?
0:08 How do we even take pictures of such nanoscopic transistors?
0:12 Well, thatās the role of the electron microscope which has
0:16 literally changed the way humanity sees the micro and nanoscopic world.
0:21 Donāt believe us?
0:22 Take this European Peacock Butterfly for example.
0:26 When we zoom in on its wing using a light microscope,
0:29 we see that itās composed of tiny overlapping scales.
0:33 But, when we zoom in using an electron microscope,
0:37 we can clearly see the shape of each scale, and zooming in further,
0:42 we see how the scales have a truly
0:45 incredible texture entirely foreign to anything that humans manufacture.
0:49 Although this wing may not be directly related
0:52 to the technology youāre familiar with, scientists and engineers
0:56 have been using electron microscopes for the past
0:59 60 years to develop smaller and smaller transistors,
1:02 and with todayās technology this microscope can zoom in millions
1:07 of times to where itās able to capture images of individual atoms.
1:13 There are two main types of electron microscopes.
1:16 The Scanning Electron Microscope or SEM is used
1:20 to see surface images like this butterfly wing,
1:24 or the bristles of a used toothbrush.
1:27 See, here are cells from your body, and all around here in yellow is bacteria.
1:33 Itās gross, but letās move on.
1:37 Scanning Electron Microscopes have a maximum resolution of around 1 nanometer.
1:42 Meaning the spacing between two adjacent features or dots
1:46 of resolvable data in an image is 1 nanometer.
1:50 The other type is the Transmission Electron Microscope or TEM which
1:54 is used to take images of structures that are inside materials,
1:59 much like an x-ray machine takes pictures of the bones inside our bodies.
2:04 For example, TEMs are used to take
2:07 the pictures of these sections of a transistor.
2:10 However, in other domains of science TEMs can
2:13 be used to take images of proteins inside mitochondria,
2:17 the powerhouse of the cell, or of nanoparticles of pure gold.
2:24 Transmission Electron Microscopes are typically more complex than
2:27 SEMs and have a resolution up to 50 picometers,
2:31 which is roughly the size of a hydrogen atom.
2:35 One quick note is that this videoās sponsor, Thermo Fisher Scientific,
2:39 provided us with a basic 3D model of one of their transmission
2:44 electron microscopes and assisted in our understanding
2:47 of the complex technology involved.
2:50 Letās first focus on the TEMs as they
2:53 are more commonly used in developing cutting-edge technology,
2:57 and later weāll provide an overview of the scanning electron microscope.
3:02 And note that thereās considerable overlap
3:04 between the engineering inside them both.
3:07 The basic idea behind a TEM is that it generates
3:11 electrons and accelerates them to around 70% the speed of light,
3:16 thus creating a beam of electrons.
3:19 Next a series of magnetic lenses focuses the electrons down to a small
3:24 area and shoots or transmits these electrons
3:27 through the specimen that weāre looking at.
3:30 Depending on the different densities and materials inside the specimen,
3:34 the electrons are scattered as they pass through it,
3:38 thereby imprinting an image of whatās inside
3:40 the specimen onto the beam of electrons.
3:43 The imprinted beam of electrons is then magnified 40 times using an objective
3:49 lens and further magnified 50,000 times using a set of projector lenses.
3:57 At this point, the imprinted image is 5 or so centimeters wide and large
4:01 enough to be captured by a high-resolution
4:04 camera sensor at the bottom of the microscope.
4:07 Weāll explore the detailed engineering in a little bit, but for now,
4:11 you might be wondering why do we have
4:14 to go through the hassle of manipulating electrons,
4:16 and why canāt we just use light?
4:19 Well, visible light is physically limited
4:22 to magnifications up to around 2000 times, and, if you try to zoom in further
4:28 the image remains blurred without revealing any more details.
4:33 On the other hand, electrons can reach
4:36 meaningful magnifications up to 2 million times.
4:40 Why then is light physically limited?
4:42 Well, letās return to this image of the European
4:45 peacock butterfly and the scales on its wings.
4:48 This image was captured with a camera,
4:51 this image was taken with a light microscope,
4:55 and these images were captured with an electron microscope.
4:59 Letās consider two features from the specimen
5:02 that are only 100 nanometers apart.
5:05 Visible light has an average wavelength of 540 nanometers,
5:08 which is larger than the distance between these two points.
5:12 Due to the physics of waves, as light hits these two features itās bent around,
5:18 thus creating a pair of propagating waves with a diffraction
5:22 pattern resulting from the interference of the two waves.
5:26 If the features are substantially closer than the wavelength of visible light,
5:30 then the diffraction pattern will make the two
5:33 features appear like a single blurred feature.
5:36 In short, visible light canāt really resolve
5:39 features that are less than 300 nanometers apart.
5:43 However, in this electron microscope,
5:45 electrons are accelerated to 70% of the speed of light and have a wavelength
5:52 of 2.5 picometers which is around
5:55 200,000 times smaller than visible lightās wavelength.
5:59 In principle, such an electron microscope could
6:02 resolve features spaced just 1 picometer apart,
6:06 but, due to the magnetic lensesā physical
6:09 limitations the real resolution is around 50 picometers,
6:12 which is enough to see individual atoms in a material.
6:17 Also, if youāre wondering about the scale of micrometers, nanometers,
6:22 and picometers, hereās a comparison of the size of each unit.
6:27 Note that there are many more details and facts that were cut from this videoās
6:31 script and thrown into the creatorās comments which
6:34 you can find in the English Canadian Subtitles.
6:38 That said, letās now dive into the complex science
6:45 and engineering behind each part of this Transmission Electron Microscope.
6:53 Weāll begin at the top with a device
6:56 called a field emission source which generates free electrons.
7:00 The basic principle is that negatively charged
7:03 electrons are attracted to positive electric fields.
7:07 Here we have a tungsten crystal needle,
7:10 and below is a ring called the extractor.
7:13 This extraction ring is connected to positive 5 thousand volts,
7:17 and as a result the negatively charged electrons
7:20 in the tungsten are pulled towards the extractor.
7:24 The electric fieldās effect on the electrons
7:27 is amplified by the sharply pointed tungsten crystal,
7:30 which is only a few nanometers wide,
7:32 and as a result the electrons are freed from the tungsten.
7:37 The next step is to accelerate them to 70% the speed of light.
7:41 To do this we use a series of metal rings which are
7:45 graduated to be tens of thousands of volts apart from one another.
7:49 And, just like before,
7:51 these positively charged rings use electrostatics to attract the negatively
7:56 charged electrons which are accelerated through the center of the rings.
8:01 There are two key reasons for the incredible speed of the electron.
8:06 First is so they can travel through the specimen, whether it be a transistor,
8:11 protein or a crystal lattice or something else that has
8:14 been sliced to typically only 100 nanometers in thickness;
8:18 and second, as mentioned earlier,
8:21 electrons exhibit wavelike properties, and the faster they are,
8:25 the shorter the wavelength and the higher the resolution achievable.
8:29 One important detail is that when the microscope is
8:32 running and electrons are being accelerated to relativistic speeds,
8:36 vacuum pumps are used to remove all the atmospheric molecules,
8:41 thus creating a vacuum, similar to the vacuum of outer space.
8:45 This is because incredibly fast-moving electrons
8:48 will scatter in random directions as they
8:51 collide with air molecules and thus ruin the images of the specimen.
8:56 Now that we have a beam of electrons,
8:59 weāll explore the magnetic lenses of which there are essentially three sets:
9:04 the condenser, the objective, and the projector.
9:08 The role of the condenser magnetic lenses is to focus
9:12 the electrons from the source and project them onto
9:15 the sample so that they illuminate an area the size
9:18 of a micrometer to several nanometers depending on the desired magnification.
9:24 Additionally, the microscope uses apertures,
9:26 or holes placed in the path of the beam to filter out
9:31 any electrons that are fanning too far from the center of the column,
9:36 or optical axis, resulting in electrons more parallel
9:39 to one another before they hit the specimen.
9:43 The specimen is placed on a holder which
9:45 is inserted through an airlock into the vacuum chamber.
9:49 To see different aspects of the specimen such as the crystal lattices,
9:53 the holder can move, or translate the specimen in all three directions,
9:58 X,Y, and Z, and rotate the specimen along the X-axis,
10:03 and with some holders, also the Y-axis.
10:07 With this we can get images exactly perpendicular
10:11 to the features such as these transistors inside.
10:15 The incredibly small beam then hits the specimen
10:19 composed of different elements and densities of materials,
10:22 thus scattering the electrons in different ways thereby
10:26 imprinting an image on the transmitted electron beam.
10:30 The next lenses, the objective and a series of four projector lenses,
10:35 are used to resolve and magnify the miniscule image imprinted
10:39 into the electron beam up to a width of a few centimeters.
10:45 This process is separated into two parts.
10:48 First the objective lensā often considered
10:51 the heart of the microscopeā magnifies
10:54 the image by 40 times and its optical aberrations define the final resolution.
11:01 Then the projector lenses magnify the image the rest of the way by 50,000 times.
11:07 What are optical aberrations and why is
11:11 2 million times the typical maximum magnification?
11:14 Well, letās look at this image of 962 blurry atoms of gold.
11:20 With todayās technology, the TEMās ability to resolve the smallest features
11:25 is not limited by the electrons in the beam,
11:29 but rather by the lenses and the aberrations and distortions that they
11:33 add to the image-imprinted electron beam after it has been magnified.
11:38 There are a few main types of aberrations such as spherical and chromatic,
11:43 which we wonāt explore further,
11:45 but the main idea is that perfectly controlling a beam of electrons is
11:50 far from trivial and the aberrations add
11:54 blurriness and impede resolution after the magnification.
11:58 The projector lenses magnify what has
12:01 already been magnified by the objective lens, including the added aberrations,
12:05 and this second magnification adds its own aberrations afterwards.
12:10 Therefore, a considerable amount of science and engineering is
12:14 dedicated to reducing the aberrations introduced by the objective lens,
12:19 as that is what ultimately limits
12:22 the sub-nanometer scale resolution of the microscope.
12:26 One thing youāre probably wondering is
12:29 why these magnetic lenses look nothing like
12:31 microscope or camera lenses and how do
12:34 magnetic lenses operate on fast moving electrons?
12:37 Well, inside the lens is a coil of copper wire surrounded by an iron housing.
12:44 When a current is run through these coils, a magnetic field is produced.
12:49 This magnetic field is then routed through the iron
12:52 to the pole pieces where itās channeled into an optical column.
12:57 These magnetic fields are then used to change the trajectory
13:01 of the electron by bending the electrons towards the center,
13:05 or optical axis, in a shrinking helical direction.
13:09 The physics at play is the Lorentz Law.
13:12 To summarize, the force on the electron is equal to its charge, Q,
13:18 times V or the electronās velocity vector crossed with B,
13:23 the magnetic field vector.
13:25 In short, if the electron were to have a velocity away from the optical axis,
13:30 it would be forced by the magnetic field down towards the center.
13:36 However, if the electron were traveling perfectly
13:38 down the center along the optical axis,
13:41 it wouldnāt experience any Lorentz force from the magnetic
13:45 fields and would just continue down the center.
13:49 As a result, the magnetic lenses act as convex or converging lenses,
13:54 focusing all the electrons down to a focal point.
13:58 As the electrons continue their trajectory past the focal point and expand,
14:03 they produce a magnified image.
14:06 This magnification depends on the strength of the magnetic fields,
14:10 the position of the lenses, and the position of the detectors and cameras.
14:15 Letās move further down the microscope
14:17 and explore how we turn electrons into images.
14:21 There are two separate systems.
14:23 First, we have a phosphorescent screen which has a special coating that glows
14:28 when electrons hit it and a camera is used to view the screen.
14:33 This system is used to align the microscope
14:36 and provide an overview of the specimen.
14:38 When youāre ready to capture a high-resolution image,
14:41 the phosphorescent screen moves out of the way,
14:45 and the image is captured using the second system with a more
14:49 sensitive CMOS camera that has a higher resolution and dynamic range.
14:53 The purpose of having two systems is
14:56 that the phosphorescent screen and camera is
14:58 used to ensure that the electron beam and magnetic lenses are set up properly,
15:03 as an incorrectly focused beam could damage the sensitive CMOS camera.
15:08 Weāve covered many key parts of the microscope,
15:11 but there are other pieces of equipment
15:13 and modules that provide additional features.
15:17 For example, there are X-Ray detectors,
15:20 energy filters, phase plates, monochromators, multipole correctors,
15:24 mechanisms to hold and adjust apertures, water cooling for the magnetic lenses,
15:30 tons of circuitry to control the magnetic lenses and the field emission source,
15:36 vacuum pumps, power supplies, and much more.
15:40 Additionally, the entire microscope sits
15:43 on air cushions to remove external vibrations.
15:46 Undoubtedly, this microscope represents an incredible
15:49 amount of science and engineering, and weāre thankful to this videoās sponsor,
15:55 Thermo Fisher Scientific, for allowing us to look inside.
15:59 In addition to electron microscopes, Thermo Fisher also makes a wide range
16:04 of laboratory equipment such as centrifuges, incubators,
16:08 xāray and mass spectrometers,
16:10 and in fact they make PCR systems that can be used to test for Covid 19.
16:17 Undeniably, Thermo Fisher products are some of the backbones
16:20 of scientific research in labs across the world.
16:24 Thermo Fisher isnāt sponsoring this video because they
16:27 want you to buy a multi-million-dollar electron microscope,
16:30 but rather, just like us at Branch Education,
16:34 they believe that the future of humanity lies
16:37 in the hands of scientistsā and engineersā abilities to discover,
16:41 innovate, and engineer solutions to the problems that face humanity.
16:46 If youāre pursuing a career in science or engineering,
16:49 take a look at Thermo Fisher Scientific.
16:52 You too could work on creating
16:55 the tools that propel science and engineering forward.
16:58 Now that we understand the transmission electron microscope,
17:02 letās look at the Scanning Electron Microscope
17:05 or SEM which Thermo Fisher Scientific also manufactures.
17:10 The main idea is that, instead of illuminating an area
17:13 of a specimen and imprinting the image all at once,
17:17 with a SEM we create a focused spot,
17:20 and scan this spot across the object weāre trying to magnify.
17:24 These electrons then bounce off, and, in the process,
17:29 create secondary electrons, back-scattered electrons and X-Rays,
17:32 which we measure to get details
17:35 as to the surface topology and chemical composition.
17:39 For example, this process was used to create these images of the butterfly wing,
17:44 or of this salt crystal.
17:47 The issue with SEM is that it only takes
17:50 images of the surfaces of materials and the resolution is
17:54 limited by how small we can create the focused spot
17:57 and by how deep the electrons penetrate into the sample,
18:01 or the so-called interaction volume.
18:03 The practical resolution is typically around 1 nanometer.
18:08 Additionally, a useful variation of the Transmission Electron
18:12 Microscope thatās worth mentioning is called an STEM,
18:16 where the S is for scanning.
18:18 This microscope is similar to the TEM, but like the SEM,
18:22 we focus the beam into a spot and then
18:25 use deflection coils to scan the spot through the specimen.
18:28 The benefit of STEM is that it has a different mechanism
18:33 for creating image contrast and, when paired with an x-ray detector,
18:38 is capable of elemental analysis of the sample.
18:42 More expensive TEMs typically have the optical elements
18:45 and circuitry to perform both TEM and STEM,
18:49 and the user can toggle between the two modes.
18:53 Weāre sure you have many questions; feel free to put them in the comments below,
18:59 and weāll try to answer them in the top pinned comment.
19:02 Also, one of the scientists from Thermo Fisher who works
19:06 on these microscopes and helped us to research and write this script,
19:10 has written the creatorās comments with loads of additional information,
19:13 so take a look at them in the English Canadian Subtitles.
19:18 We believe the future will require
19:20 a strong emphasis on engineering education and weāre
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19:36 This is Branch Education, and we create 3D animations that dive deeply
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19:51 Thanks for watching to the end!