What is biometry in ophthalmology?

Biometry is the application of mathematics to biology, specifically in ophthalmology, it refers to the calculation of intraocular lens power.

What factors are measured in biometry?

Key factors include axial length, central corneal power, anterior chamber depth, lens thickness, effective lens position, and white-to-white width.

What are the types of biometers?

There are two main types: ultrasound biometers (contact and immersion) and optical biometers.

What is the significance of axial length measurement?

Axial length measurement is crucial as errors can lead to significant postoperative refractive errors.

How does ultrasound biometry work?

It works on the principle of the piezoelectric effect, where mechanical deformation generates ultrasonic waves that reflect off eye structures.

What is the difference between contact and immersion biometers?

Contact biometers touch the cornea directly, while immersion biometers use a shell to avoid corneal compression.

What are common sources of error in biometry?

Common errors include corneal compression, misalignment of the probe, and variations in eye anatomy.

How does sound velocity affect measurements?

Sound travels at different velocities in various eye media, affecting the accuracy of distance calculations.

What is the role of gain in ultrasound biometry?

Gain amplifies the ultrasound signal, but too much gain can introduce noise and reduce resolution.

Why is proper alignment of the probe important?

Proper alignment ensures accurate measurements by maximizing the amplitude of reflected sound waves.

A SCAN BIOMETRY | Principles, contact and immersion biometry |

00:39:49

https://www.youtube.com/watch?v=CrUJJDqDwPA

Summary

TLDRIn this lecture, Dr. Amrit discusses ultrasound biometry, a critical method in ophthalmology for calculating intraocular lens power during cataract surgery. The lecture outlines the prerequisites for accurate biometry, including measurements of axial length, corneal power, and anterior chamber depth. It highlights the importance of precision, as errors in these measurements can lead to significant postoperative refractive errors. The types of biometers are explained, focusing on ultrasound biometers (contact and immersion) and their operational principles based on the piezoelectric effect. The lecture also addresses common sources of error, the impact of sound velocity on measurements, and the significance of proper probe alignment. Overall, the session emphasizes the need for accurate biometry to meet rising patient expectations for refractive outcomes post-surgery.

Takeaways

👁️ Biometry is crucial for calculating intraocular lens power.
📏 Accurate axial length measurement is vital to avoid refractive errors.
🔍 Ultrasound biometers use sound waves for measurements.
⚖️ Immersion biometers prevent corneal compression, improving accuracy.
📊 Errors in measurements can significantly affect surgical outcomes.
🔧 Proper alignment of the probe is essential for reliable results.
📈 Gain settings can amplify signals but may introduce noise.
🧪 Different eye media affect sound velocity and measurement accuracy.
📝 Understanding the types of biometers helps in choosing the right tool.
💡 Patient expectations for refractive outcomes have increased.

Timeline

00:00:00 - 00:05:00
Dr. Amrit introduces the topic of ultrasound biometry in ophthalmology, explaining that biometry applies mathematics to biology, particularly for calculating intraocular lens (IOL) power. He emphasizes the importance of accurate IOL power calculation for achieving excellent refractive outcomes in cataract surgery, which now aims for no refractive error post-surgery.
00:05:00 - 00:10:00
The prerequisites for IOL power calculation include measuring axial length, central corneal power, anterior chamber depth, lens thickness, effective lens position, white-to-white width, and corneal thickness. Errors in these measurements can lead to significant postoperative refractive errors, with specific percentages attributed to each measurement error.
00:10:00 - 00:15:00
The normal range for axial length is discussed, highlighting that longer eyes are more forgiving of measurement errors, while shorter eyes are less forgiving. The importance of obtaining data from both eyes is emphasized, particularly if there is a significant inter-eye difference in axial length.
00:15:00 - 00:20:00
Dr. Amrit explains the two types of biometers: ultrasound and optical. Ultrasound biometers can be contact or non-contact (immersion), while optical biometers use light. He notes that ultrasound biometers do not measure corneal power directly, unlike optical biometers, which integrate this measurement.
00:20:00 - 00:25:00
The working principle of ultrasound biometers is based on the piezoelectric effect, where mechanical deformation generates electricity. The ultrasound probe sends waves that reflect off various eye structures, and the machine calculates distances based on the time taken for these waves to return, using the formula distance = speed x time.
00:25:00 - 00:30:00
Different types of ultrasound biometers are discussed, including contact and immersion methods. The immersion method avoids corneal compression, providing more accurate readings. The importance of proper alignment of the probe and the quality of the interface for accurate readings is emphasized.
00:30:00 - 00:39:49
Common errors in ultrasound biometry include corneal compression, misalignment of the probe, and issues with the quality of the ocular interface. Dr. Amrit discusses how to identify and correct these errors, as well as the advantages of immersion scans over contact scans, particularly in reducing technician dependency and improving accuracy.

Mind Map

Video Q&A

What is biometry in ophthalmology?
Biometry is the application of mathematics to biology, specifically in ophthalmology, it refers to the calculation of intraocular lens power.
What factors are measured in biometry?
Key factors include axial length, central corneal power, anterior chamber depth, lens thickness, effective lens position, and white-to-white width.
What are the types of biometers?
There are two main types: ultrasound biometers (contact and immersion) and optical biometers.
What is the significance of axial length measurement?
Axial length measurement is crucial as errors can lead to significant postoperative refractive errors.
How does ultrasound biometry work?
It works on the principle of the piezoelectric effect, where mechanical deformation generates ultrasonic waves that reflect off eye structures.
What is the difference between contact and immersion biometers?
Contact biometers touch the cornea directly, while immersion biometers use a shell to avoid corneal compression.
What are common sources of error in biometry?
Common errors include corneal compression, misalignment of the probe, and variations in eye anatomy.
How does sound velocity affect measurements?
Sound travels at different velocities in various eye media, affecting the accuracy of distance calculations.
What is the role of gain in ultrasound biometry?
Gain amplifies the ultrasound signal, but too much gain can introduce noise and reduce resolution.
Why is proper alignment of the probe important?
Proper alignment ensures accurate measurements by maximizing the amplitude of reflected sound waves.

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Subtitles

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00:00:00
hello and welcome to Insight oftalmology
00:00:03
this is Dr Amrit welcoming you to
00:00:05
another lecture today we are talking
00:00:07
about the ultrasound biometry so what is
00:00:11
biometry as the name suggests biometry
00:00:13
is the method of applying mathematics to
00:00:16
biology the term was originally used for
00:00:19
calculating the life expectancy however
00:00:22
in the field of oftalmology it deals
00:00:25
with the intraocular lens power
00:00:27
calculation the total refractive power
00:00:30
power of the eye primar depends upon the
00:00:32
coral
00:00:33
power it depends upon the lens power the
00:00:39
media and the axial length calculation
00:00:42
the present day cataract surgery doesn't
00:00:44
just aim at removing of the removal of
00:00:47
the cataractous lens but also at the
00:00:50
implantation of the intraocular lens and
00:00:53
giving the patient excellent refractive
00:00:55
outcomes all this is going to depend
00:00:57
upon our calculation of IAL power lens
00:01:01
Power Media and the axial length with
00:01:05
the technological advancement in the
00:01:07
cataract surgery and introduction in the
00:01:09
premium iol patients expectations have
00:01:13
actually risen and therefore now they
00:01:15
aim at getting no refractive error
00:01:17
following the cataract surgery any
00:01:20
refractive error is no longer tolerated
00:01:23
and therefore it's very very important
00:01:25
that we carry out our I power
00:01:27
calculation and biometry accurately
00:01:31
let us consider what are some of the
00:01:33
prerequisites for iul power calculation
00:01:36
in biometry we measure the axial length
00:01:39
we measure the central Coral power we
00:01:42
also measure what is known as the
00:01:44
anterior chamber depth apart from this
00:01:47
other things which are also measured are
00:01:49
the lens thickness the effective lens
00:01:52
position also know known as the ELP then
00:01:55
we have the white to white width then we
00:01:58
have Coral thickness is known as Petry
00:02:01
now let us discuss how much these
00:02:03
factors account as the sources of errors
00:02:06
in the intraocular lens power
00:02:08
calculation the first one is the
00:02:11
prediction of the effective lens
00:02:13
position and if you actually observe
00:02:15
this contributes the maximum percentage
00:02:17
responsible for inaccuracy in the I
00:02:20
power
00:02:21
calculation then we have the
00:02:22
post-operative refraction then we have
00:02:25
the axial length measurement errors
00:02:27
accounting for 17% of the ER inesis then
00:02:31
we have the keratometry measurements a
00:02:35
01 01 mm error in the axial length
00:02:39
calculation in an ie which has an
00:02:42
average axial length will lead to a post
00:02:45
operative refractive error of about 0.25
00:02:48
diopters so what you can say over here
00:02:51
is that one mm error in the axle length
00:02:56
will lead to about 2.5 diopters of of
00:03:00
postoperative refractive error in an i
00:03:02
which has normal or average axile length
00:03:06
next if you consider the coral power
00:03:08
errors if you do a Coral power error of
00:03:11
about one diopter in an i with average
00:03:14
length the post operative refractive
00:03:16
error would be about one diopter okay so
00:03:20
remember a 1 mm error in the axle length
00:03:23
will lead to about 2.5 diopters of
00:03:25
postoperative refractive error and in
00:03:27
one diopter error in the coral power
00:03:30
will lead to postoperative refractive
00:03:32
error of about one diopter okay remember
00:03:36
that let us talk about the normal axial
00:03:39
length the normal range of axial length
00:03:41
is about 22 to 24.5 mm and the average
00:03:45
is 23.5 mm this is important to know
00:03:50
because in eyes which have nor uh longer
00:03:53
Axel length than the average these eyes
00:03:56
are much more forgiving for example if
00:03:58
you take an eye which is about 30 mm
00:04:01
long in that IE a 1 mm error in the axle
00:04:06
length will lead to a postoperative
00:04:08
error of about 1.75 diopters compared to
00:04:12
the 2.5 diopter error that occurs in an
00:04:15
average length eye okay smaller eyes are
00:04:18
least forgiving for example in an ie
00:04:21
which is about 20 mm long and there is
00:04:24
an error of 1 mm the postoperative
00:04:27
refractor error is going to be much more
00:04:29
it is about 3.75 de opter which is much
00:04:32
greater than the 2.5 de opter error
00:04:34
which was occurring in a normal axal
00:04:36
length IE okay so what you can remember
00:04:39
is that the errors are more in smaller
00:04:41
eyes compared to the average eye
00:04:43
compared to the longer eyes and the
00:04:45
longer eyes are the most
00:04:48
forgiving now whenever we are doing axil
00:04:51
length calculation you always have to
00:04:53
obtain the data from two eyes and if the
00:04:56
inter eye difference of the axle length
00:04:59
is greater than3 mm then you have to be
00:05:03
suspicious we'll talk about this in a
00:05:05
while first let us try to discuss now
00:05:08
the types of biometers which are
00:05:10
available based on the energy that
00:05:12
you're using we have two types of
00:05:14
biometers we have an ultrasound biometer
00:05:17
and an optical biometer in ultrasound
00:05:20
biometers we using the sound waves and
00:05:22
in Optical biometers we are using what
00:05:24
is known as the light source okay light
00:05:27
as a source of energy now ultrasound
00:05:30
biometers again are of two types so we
00:05:32
have contact biometers in which the
00:05:35
probe touches the cornea directly and we
00:05:38
have a non-con biometer in which the
00:05:40
probe doesn't touch the cornea directly
00:05:43
instead the probe is actually immersed
00:05:45
in a scal shell which is placed on the
00:05:47
cornea and therefore this type of
00:05:50
ultrasound biometry is also known as the
00:05:52
immersion or non cont biom meter
00:05:57
okay let us see what are the types of
00:05:59
optical biometers which are available so
00:06:01
we have those which are based on the
00:06:03
principle of partial coherence
00:06:06
interferometry that is the I Master 500
00:06:09
we have those which are based based on
00:06:11
the optical low coherence reflector
00:06:14
metry like the lensar 900 OA 2000 gal G6
00:06:19
then we have swept Source OC like the I
00:06:22
master 700 now for the purpose of this
00:06:25
video we shall be limiting ourselves to
00:06:27
the ultrasound biometers like the
00:06:30
contact and the immersion biometer a
00:06:33
very important point that we must
00:06:35
remember is that the ultrasound
00:06:37
biometers doesn't uh really measure the
00:06:41
coral power okay unlike the optical
00:06:44
biometers so whenever you do an optical
00:06:46
biometry you don't need to really
00:06:48
measure the coral power separately the
00:06:50
biometer does it for you right whereas
00:06:53
when you do an ultrasound biometry you
00:06:55
actually need to separately calculate
00:06:57
the coral power using a keratometer or a
00:07:02
topographer now we have a series on
00:07:04
topography available on our channel in
00:07:07
which the first video is on the basics
00:07:08
of coral topography then we have uh on
00:07:11
the maps and then we have on how to read
00:07:14
a coral tomography print out all right
00:07:16
so you can check the links which are
00:07:18
present in the description
00:07:20
box next let us talk about how the
00:07:23
ultrasound biometers actually work so
00:07:25
they're basically working on the
00:07:27
principle of piso electric effect or p
00:07:29
Electric effect however you want to
00:07:31
pronounce it now the Greek word pison
00:07:35
basically stands for to squeeze or to
00:07:39
compress okay and piso electric effect
00:07:42
basically means mechanical deformation
00:07:45
of a piso electric material always leads
00:07:48
to generation of electricity so there
00:07:51
are certain materials like the quads
00:07:54
okay and what's going to happen in these
00:07:56
materials that whenever you apply Force
00:07:58
to deform these materials either squeeze
00:08:00
them or compress them is going to lead
00:08:03
to generation of electricity and also
00:08:06
vice versa is also true so what I mean
00:08:08
to say is if you apply electricity to
00:08:11
such materials it is going to lead to
00:08:13
the uh mechanical deformation of these
00:08:16
materials right so this is known as the
00:08:19
piso electric effect now this is
00:08:21
important because the ultrasound probe
00:08:24
actually is made up of these piso
00:08:26
electric crystals and these piso
00:08:28
electric crystals
00:08:30
they whenever there's application of
00:08:32
external electric energy to this probe
00:08:35
they will start vibrating they will get
00:08:37
deformed and as they get deformed and
00:08:39
they start vibrating they will generate
00:08:42
these ultrasonic waves right so these
00:08:45
ultrasonic waves are now going to travel
00:08:47
inside the eye and now they will get
00:08:50
reflected from the various structures
00:08:52
that these waves are going to encounter
00:08:54
like the cornea lens avitus retina and
00:08:58
the Scara and then then they will be
00:09:00
reflected back in the opposite direction
00:09:02
to the ultrasound machine and now since
00:09:05
the machine is again getting some sort
00:09:07
of energy the fiso electric crystals are
00:09:09
going to again vibrate and now they are
00:09:12
going to give us what is known as the
00:09:14
echo or these spikes right now these
00:09:17
Echoes and spikes are going to be
00:09:18
recorded on the screen right so you can
00:09:21
see clearly how the ultrasound works on
00:09:23
the principle of piso
00:09:25
electricity all right so you can see a
00:09:28
probe over here so this probe is going
00:09:30
to continuously uh this probe sorry is
00:09:32
going to send these ultrasonic waves now
00:09:35
one important point that you should know
00:09:37
is that these waves are traveling at a
00:09:39
particular velocity okay the sound has
00:09:42
this velocity U particular velocity in
00:09:45
various media in the eye right and these
00:09:48
waves are taking a particular time
00:09:50
period for traveling towards the object
00:09:53
and coming back towards from the object
00:09:55
to the probe right the machine is
00:09:58
basically going to operate in this pulse
00:10:01
system now pulse system basically means
00:10:04
that the probe is vibrating for some
00:10:07
time it's pulsating for some time and
00:10:09
then it takes a pause right for a few
00:10:11
micros seconds so that all these
00:10:13
returning Echoes can be received by the
00:10:16
probe tips and it is that it is during
00:10:18
that time that these signals are going
00:10:20
to be converted into spikes or Echoes
00:10:23
right now
00:10:25
usually the audible frequency to a human
00:10:28
ear is about about 20 to 20,000 Hertz
00:10:31
right however you can see the frequency
00:10:34
which a probe uses is about 10 mahz
00:10:38
right so it's a really high frequency
00:10:41
and the advantage of high frequency is
00:10:43
that it offers higher resolution all
00:10:46
right now the sound is going to travel
00:10:49
at a particular velocity within the eye
00:10:51
and we know that the waves are coming
00:10:52
back towards the probe they're taking
00:10:54
some time to go towards the object and
00:10:57
some time to come back towards the probe
00:10:59
the machine is going to calculate all
00:11:01
that time and once it has calculated
00:11:04
that time it is going to use the formula
00:11:08
that is speed into time equals distance
00:11:11
and it is using by using this formula
00:11:13
the machine is going to calculate the
00:11:14
various distances like the axal length
00:11:18
anterior chamber depth and the length
00:11:21
thickness okay so I hope you understood
00:11:23
how the axle length is calculated by the
00:11:26
machine all right now let us let talk
00:11:29
about some other principles of the
00:11:31
ultrasound you should know that the
00:11:34
sound usually travels faster in solids
00:11:37
compared to liquid okay and therefore
00:11:40
the velocity of the sound waves as
00:11:42
they're going to travel within the eye
00:11:44
is constantly changing in an a scan
00:11:47
biometer the sound is traveling through
00:11:50
the solid Gia then it has to travel in
00:11:53
the liquid Vitus then it has to travel
00:11:56
again in the solid lens again it travel
00:11:59
travels in the solid or the liquid or
00:12:01
you can say semif fluidic witus again it
00:12:04
travels in the retina choid Scara and
00:12:07
finally into the orbital tissue and
00:12:09
therefore we can say that the velocity
00:12:11
of the sound waves within the eye is
00:12:13
also constantly
00:12:16
changing right so you can observe over
00:12:18
here the speed of the sound waves within
00:12:21
the cornea is about 1641 m/s in lens
00:12:25
again it is somewhat similar in the
00:12:27
Aquis humor and in the humor because
00:12:29
they are more liquidy compared to the
00:12:31
cor and the lens and therefore the speed
00:12:33
over here is about 15 32
00:12:36
m/s now usually uh the machine averages
00:12:40
these values and therefore the average
00:12:42
sound velocity in a normal fake ey is
00:12:45
about 1550
00:12:48
m/s okay now the cornea is not routinely
00:12:51
factored in because the thickness of the
00:12:53
cornea is really less about 0.5 mm and
00:12:57
therefore the cornea uh the velocity of
00:12:59
the sound in the Cora is Lally not
00:13:00
factored in now the average sound
00:13:03
velocity in an eye which does not have
00:13:05
the lens that is an earth fic eye will
00:13:08
come to about 1532
00:13:11
m/s okay now what about the average
00:13:13
sound velocity in a pseudo ey now we
00:13:16
know that pseudo FIA means presence of
00:13:18
an intraocular lens now intraocular
00:13:21
lenses again could be of various
00:13:24
materials and therefore the average
00:13:27
sound velocity in a pseudo fic eye is is
00:13:29
going to be 1532 m/s plus or minus the
00:13:34
correction factor for that intraocular
00:13:37
material okay so we'll talk about the
00:13:38
correction factors also in a
00:13:41
while now a very important point that we
00:13:44
must all know is that within the eye we
00:13:47
have various interfaces that means for
00:13:49
example the air and the cornea is one
00:13:52
interface the cornea and the Aquis is
00:13:54
one interface between the Aquis and the
00:13:56
lens is another interface and then again
00:13:59
between the lens witus witus retina
00:14:01
retina and Scara there are different
00:14:03
different interfaces right so the echo
00:14:05
are received back into the probe after
00:14:08
being reflected from these interfaces
00:14:11
and these Echo are going to be converted
00:14:13
by the biometer into various spikes
00:14:15
which are arising from the Baseline as
00:14:17
you can see over here the greater is the
00:14:20
difference between the two Media or at
00:14:22
each interface for example between the
00:14:24
Aquis and the lens the greater is the
00:14:27
difference in these two media at the
00:14:29
interface the stronger is going to be
00:14:32
the spike and the stronger is going to
00:14:33
be the echo right and if the interface
00:14:36
difference is less the echo is going to
00:14:38
be weaker and the strong uh the strength
00:14:42
and the weakness of the echo basically
00:14:43
is represented in the form of amplitude
00:14:46
Okay so what you're doing in a biometer
00:14:49
is an a scan that is and over here a
00:14:52
basically stands for the amplitude
00:14:55
representation of the echo along the
00:14:57
path and it is a onedimensional
00:14:59
representation remember that all right
00:15:02
so now let us talk about these various
00:15:04
types of ultrasound biometers so we have
00:15:06
the contact biometer and the immersion
00:15:08
or non- cont biometer so let's see first
00:15:12
about the contact a scan also known as
00:15:15
the applanation a scan or biometry now
00:15:18
the term applanation I personally don't
00:15:20
like to call it that way because ideally
00:15:23
speaking you're not supposed to
00:15:24
applanate when carrying out a contact a
00:15:26
scan as well you're just supposed to
00:15:28
touch the probe to the patient's eye
00:15:30
okay compression or any sort of
00:15:32
applanation will lead to uh inaccurate
00:15:35
readings in contact biometry all right
00:15:38
the patient could be seated or the
00:15:40
patient could be lying down Supine
00:15:42
position you have to instill a topical
00:15:44
anesthetic solution and what you have to
00:15:47
do is you have to give the patient a
00:15:48
fixation Target like this okay and then
00:15:52
the examiner has to gently touch the
00:15:54
cornea without causing any indentation
00:15:58
okay and as you do so there will be
00:16:00
generation of these spikes as you can
00:16:02
see right the first spike is coming from
00:16:05
as you can see from the cornea and the
00:16:07
probe since the probe is in contact with
00:16:09
the cornea you get the first Spike then
00:16:11
you get one Spike from the anterior
00:16:13
surface of the lens then you get another
00:16:15
from the posterior surface of the lens
00:16:17
then you get one Spike from the retina
00:16:18
and one from the Scara okay let's talk
00:16:21
about that now over here the patient
00:16:23
could be sitting or the patient could be
00:16:25
lying down but make sure that the plane
00:16:28
of the iris is parallel to the floor
00:16:30
there should be no pillows or or no
00:16:32
headrest below the patient okay and
00:16:34
obvious and always make sure that you
00:16:36
give the fixation Target to the patient
00:16:39
when carrying out the contact bio
00:16:41
contact biometry make sure that you hold
00:16:45
the probe from The Wire okay this
00:16:46
actually reduces the compression force
00:16:49
on the cornea if you're going to
00:16:51
directly hold the probe from the uh end
00:16:54
of the probe it there are more chances
00:16:56
that you might actually compress the
00:16:58
cornea okay always make sure you give
00:17:00
the accurate
00:17:02
or adequate Target like patient can use
00:17:05
his own thumb or you can give a fixation
00:17:07
light as a Target and even the a scan
00:17:09
probe comes with a fixation light
00:17:11
usually it is red in color so you can
00:17:13
ask the patient to look towards the
00:17:15
light all right now a high quality
00:17:18
contact a scan of a fake eye basically
00:17:21
consists of five high amplitude spikes
00:17:24
okay remember now you might say there
00:17:26
are so many spikes over here yes they
00:17:28
are but what is important for us are the
00:17:31
high amplitude spikes so we have five
00:17:34
high amplitude spikes you can see the
00:17:36
first one which is coming from the
00:17:38
cornea and the probe together because
00:17:41
the probe and cornea are in touch with
00:17:42
each other then we have the one which is
00:17:45
coming from the anterior lens then we
00:17:47
have one coming from the posterior lens
00:17:49
then we have the spike which is coming
00:17:51
from the retina and Spike which is
00:17:53
coming from the Scara so all these are
00:17:55
high amplitude spikes then of course we
00:17:57
have smaller spikes which are coming
00:17:59
from the orbital tissues another thing
00:18:01
you should know note is that these all
00:18:04
these Spikes have to rise steeply from
00:18:07
the surface especially the retinal Spike
00:18:09
if you see it has to make this 90° angle
00:18:13
also there should be good resolution and
00:18:15
these spikes should be separate there
00:18:17
should be no intermixing of the retina
00:18:19
and the Scara spikes so that is very
00:18:21
important so Spike height or amplitude
00:18:24
is what provides us the information on
00:18:27
the quality about the quality of the a
00:18:30
scan and therefore since we are
00:18:32
basically relying our biometry on the
00:18:34
amplitudes and therefore this type of
00:18:36
biometry is known as an a scan or an
00:18:39
amplitude scan so I hope that is clear
00:18:42
all right so now let us talk about the
00:18:44
immersion or non- cont biometry now over
00:18:47
here what you can see is that there is a
00:18:50
sort of a shell that is placed on the
00:18:52
cornea and this shell is known as the
00:18:54
Prager shell or you can call it as a
00:18:56
Hansen shell the purpose of a
00:18:59
compression uh sorry the purpose of an
00:19:01
immersion biometer is that it avoids any
00:19:05
Coral compression because you can see
00:19:07
there's a there's some sort of distance
00:19:08
between the probe and the cornea over
00:19:11
here okay and therefore you're going to
00:19:13
see many spikes here you are going to
00:19:15
see a spike that is separately coming
00:19:17
from the probe then you see a corneal
00:19:19
Spike the corneal Spike seems to be
00:19:21
having these two peaks then you have an
00:19:24
anterior lens spike a posterior lens
00:19:26
Spike then you have a retina Spike and a
00:19:28
scler Spike and of course the orbital
00:19:30
Spike okay so in this also you make the
00:19:34
patient lie down spine make sure there's
00:19:36
no pillow underneath this and also you
00:19:39
have to again put anesthetic drops okay
00:19:42
make sure you avoid Coral compression
00:19:44
obviously this will be avoided in case
00:19:46
of this immersion biom meter ask the
00:19:48
patient to fix it align the probe with
00:19:50
the optical axis and now you have to
00:19:52
observe the various Echo and the spikes
00:19:55
which are observed okay so over here the
00:19:58
scleral shell is known as the Hansen or
00:20:00
the Prager shell and it is usually
00:20:02
filled up with saline you have to make
00:20:04
sure that no air bubbles enter the
00:20:06
saline and the probe should be immersed
00:20:10
in the saline and it should be about a
00:20:12
distance of about 5 to 10 mm away from
00:20:15
the cornea that is very very
00:20:18
important let us try to observe the
00:20:20
various waves that we see in an
00:20:22
immersion scan of a fake ey so over here
00:20:25
instead of five you're going to see six
00:20:27
waves so the first one is coming from
00:20:29
the probe the second one is from the
00:20:31
cornea then you have from the anterior
00:20:34
surface of the lens the posterior
00:20:35
surface of the lens the the retina and
00:20:38
the Scara of course there are some lower
00:20:41
amplitude waves as well these might be
00:20:43
coming from the vitus degeneration or
00:20:45
structures present within the vitus then
00:20:48
over here you have smaller wavelets
00:20:50
which are coming from the orbital fat
00:20:52
now two important things that you have
00:20:54
to remember which differentiates it from
00:20:56
a contact biometer in an immersion scan
00:20:59
you have the separate probe and coral
00:21:01
spikes the coral Spike over here
00:21:04
demonstrate two peaks okay you can see
00:21:05
this is bit so the first one is actually
00:21:08
coming from the epithelium and the
00:21:09
second one is coming from the
00:21:11
endothelium and you have to also note
00:21:13
that these two spikes which are coming
00:21:15
the two peaks of the coral Spike they
00:21:18
should be of equal amplitude in any case
00:21:20
if the these are not equal they should
00:21:22
actually U raise suspicion that the
00:21:25
probe is not aligned through the coral
00:21:27
vertex alignment of the probe is really
00:21:30
really important whether we talking
00:21:32
about contact biometry or the non-con
00:21:35
biometry so let's see why that happens
00:21:38
so if you're going to align the probe
00:21:40
basically like this to the uh whenever
00:21:44
the probe is nicely aligned parall uh
00:21:47
parall to the visual Axis or coagular to
00:21:50
the visual axis what's going to happen
00:21:51
is that all the sound waves which are
00:21:53
traveling from the probes they're going
00:21:55
to be reflected and they're going to be
00:21:57
traveling back
00:21:59
to the visual axis and all of them are
00:22:00
going to be received by the probe and
00:22:03
since all the sound wave is received by
00:22:06
the probe the spike amplitude is also
00:22:08
going to be good however if the probe is
00:22:12
not aligned correctly the waves are
00:22:14
going to be incident in an oblique
00:22:15
fashion and therefore some of the Waves
00:22:17
which are reflected they're not going to
00:22:19
make to the probe and instead they're
00:22:20
going to be reflected outside and this
00:22:23
will lead to compromise amplitude or
00:22:25
compromise signal um in the a scan
00:22:28
biometry okay and therefore it is very
00:22:31
important uh that the probe is oriented
00:22:34
nicely parallel to the visual axis at
00:22:36
the coral Vortex
00:22:39
okay next point is regarding the shape
00:22:42
and smoothness of the interface okay I
00:22:45
already told you what exactly is meant
00:22:46
by interface so over here we are talking
00:22:49
about the maula for example when the
00:22:51
maula is smooth okay all the waves are
00:22:54
going to be reflected nicely parallel to
00:22:56
the visual axis and they're going to be
00:22:58
uh
00:22:59
received by the probe and therefore the
00:23:01
amplitude is going to be nice and smooth
00:23:03
okay big nice amplitude however if the
00:23:06
macula is not smooth for example if
00:23:08
there's any irregularity in the surface
00:23:10
of the interface like if there is any
00:23:13
macula EMA if there's pigment epithelial
00:23:15
Detachment or if there's any epiretinal
00:23:17
membrane what is going to happen is that
00:23:19
there's also going to be reflection away
00:23:21
from the probe sometimes there might be
00:23:23
refraction of the returning sound waves
00:23:25
away from the probe and therefore a few
00:23:28
way only are going to make up to the tip
00:23:30
and therefore it lead to weaker Echoes
00:23:33
or weaker signals or low amplitude
00:23:34
spikes okay and therefore in order to
00:23:37
get a correct biometer readings it's
00:23:39
very important that you have a normal
00:23:41
maula as well all right for example over
00:23:45
here you can see this is basically a
00:23:48
good retinal spike a good retinal Spike
00:23:50
should actually rise sharply like this
00:23:53
it should be at 90°
00:23:55
angle all right now let's talk about
00:23:58
about the the concept of sound
00:24:01
absorption now we know that sound is
00:24:04
basically absorbed by everything through
00:24:06
which it passes before it travels to the
00:24:08
next interface so the greater is the
00:24:10
density of the structure through which
00:24:12
the sound is actually passing through
00:24:14
greater is going to be the amount of
00:24:16
absorption and therefore in a case of
00:24:18
extremely dense cataract like this
00:24:20
greater amount of sound energy is going
00:24:22
to be absorbed and there will be
00:24:24
attenuation of the signal that you're
00:24:25
going to get on your display okay and
00:24:28
that is a reason why in case of an
00:24:30
extremely dense cataract you're not
00:24:32
going to get really high amplitude
00:24:33
retinal spikes because the lens is going
00:24:35
to absorb most of the sound energy that
00:24:38
reaches the retinal surface okay so over
00:24:41
here you can see the waveforms are quite
00:24:44
shrunken actually you can see over here
00:24:46
multiple retinal uh multiple internal
00:24:48
spikes you don't have those classic five
00:24:51
spikes that you see and this happens
00:24:53
because of the uh various refractive
00:24:56
indexes uh which is present with within
00:24:58
the lens and the lens is also absorbing
00:25:00
most of the sound energy and therefore
00:25:02
you're not getting good amount of you're
00:25:04
not getting the proper morphology of the
00:25:06
spikes right so that is one problem that
00:25:09
can occur when you're carrying out
00:25:10
biometry in case of the uh dense
00:25:14
cataracts now this brings us to the
00:25:16
concept of gain in ultrasound so when
00:25:18
you're getting this uh dampened signals
00:25:21
because of a cataract is there a way
00:25:24
that we can amplify the signal yes you
00:25:26
can amplify the signal by increasing the
00:25:28
gain right so gain is that property
00:25:31
which is measured in DCB it is basically
00:25:33
the amplification of the ultrasound
00:25:35
signal that returns to the transducer
00:25:38
after passing through the tissue okay so
00:25:41
uh in cases of dense cataract we might
00:25:43
need to increase the gain these higher
00:25:46
gains will lead to increase amplitude it
00:25:49
increases the sensitivity and but the
00:25:51
only problem over here with increased
00:25:54
gains is that since the machine has now
00:25:56
become more sensitive there's going to
00:25:58
be more noise as well and therefore
00:26:00
you're going to suffer in terms of
00:26:02
resolution however in certain cases
00:26:05
where there is a fake here where there's
00:26:07
no lens to actually absorb you don't
00:26:09
need that much amount of signal and
00:26:11
there you can actually reduce your gain
00:26:14
so in AIC AIC patients you can actually
00:26:18
uh go for a lower gain setting now in
00:26:21
the first picture you can see the gain
00:26:22
is too high so when the gain is too high
00:26:24
the machine has become more sensitive
00:26:26
and it's picking up every random signal
00:26:28
and therefore you can see there's a lot
00:26:30
of noise over here instead of seeing two
00:26:32
two spikes one from retina one from
00:26:34
Scara you're seeing this broaden
00:26:37
thickened Spike with a flattened Peak
00:26:39
right this indicates that there is too
00:26:41
much gain so when there's too much gain
00:26:43
you're going to get a strong signal but
00:26:45
the resolution is going to be poor now
00:26:48
in such cases you have to actually
00:26:50
reduce the gain until the retinal and
00:26:53
the scar surfaces are seen as separate
00:26:55
spikes okay so if you uh reduce the gain
00:26:59
the resolution is going to be good but
00:27:01
the signal is going to be weaker okay so
00:27:03
that so you really have to decide what
00:27:06
exactly you want now ideally the retinal
00:27:09
and the scleral spike should be separate
00:27:11
and if you're carrying out an immersion
00:27:12
scan the peaks of the coral Spike that
00:27:15
is one coming from the epithelium one
00:27:17
coming from the endothelium they they
00:27:19
must also be separate if there's any
00:27:21
Fusion between these two then also it's
00:27:23
an indicator that you have to reduce the
00:27:27
uh you have to reduce the gain in order
00:27:29
to separate these two
00:27:31
peaks all right now let us talk about
00:27:34
the concept of electronic calipers or
00:27:37
the gates okay we all know what calipers
00:27:40
are so calipers are something which are
00:27:42
used to measure uh the distance between
00:27:44
two points right so electronically also
00:27:47
the machine introduces these uh Gates so
00:27:50
gates are these electronic calipers on
00:27:52
the display screen that measure between
00:27:54
the two points okay so biometers are
00:27:57
designed so that between each pair of
00:27:59
the gates a measurement is rendered for
00:28:01
example you're going to the biometer is
00:28:03
going to automatically place a gate over
00:28:05
here near the probe and the Cora then
00:28:07
it's going to place a gate where it
00:28:08
believes that the lens lens is spiking
00:28:11
uh lens anterior surface is spiking then
00:28:14
it's going to place a gate somewhere
00:28:15
near the posterior surface a gate near
00:28:17
the retina a gate near the Scara okay so
00:28:20
the biometer automatically places the
00:28:22
gate on what it believes to be the
00:28:24
central cornal Spike anterior lens Spike
00:28:26
posterior lens Spike retinal Spike so on
00:28:28
and so forth right and it is also
00:28:30
programmed to measure the distance
00:28:32
between each of these pairs at a given
00:28:35
velocity right so the ultrasound is
00:28:38
actually going to place these Gates
00:28:39
automatically and also it is at this
00:28:41
Gates that it is going to record the
00:28:43
time taken for the sound to travel from
00:28:45
one point to another and then the
00:28:47
machine is going to use this uh formula
00:28:50
distance equal to Velocity into time and
00:28:52
it's going to calculate the various
00:28:53
distances between these Gates and of
00:28:56
course we know how the velocity at
00:28:58
various parts of the uh I is Right
00:29:02
similarly also know about the average
00:29:04
sound velocities in the fake eye a fic
00:29:07
eye and in the pseudo fic eye as well
00:29:11
now if you know that the average sound
00:29:12
velocity in fake or fic and pseudophakic
00:29:15
ey is you should also know that there
00:29:17
are various modes which are present
00:29:19
within the biometer machine so in these
00:29:21
modes you can actually choose whether
00:29:23
you are dealing with a fake person that
00:29:25
is normal person or you're dealing with
00:29:27
an earth pic person or whether you are
00:29:29
doing a biometry in a case of a patient
00:29:33
who already has an i inside him so that
00:29:36
is known as a pseudo fic eye right so
00:29:39
again within the pseudo fic eye there
00:29:40
can be various settings which can be
00:29:42
available so there might be a setting
00:29:44
for the material that means you might be
00:29:47
able to choose whether the material is
00:29:48
PMA acrylic or the Silicon right so now
00:29:52
when you carry out a biometry in case of
00:29:54
pseudo gu you might actually be able to
00:29:56
see a lot of these spikes these spikes
00:29:59
basically are known as reverberation
00:30:00
artifact and these are more prominent
00:30:03
when the intraocular lens is basically
00:30:05
of pmma variety right so a pmma lens is
00:30:09
going to or an interocular lens is going
00:30:11
to give more reverberation artifacts
00:30:14
compared to a foldable I which is made
00:30:16
up of usually acrylic or the uh silicon
00:30:19
right so you can see the second picture
00:30:22
there is a foldable or I which is used
00:30:24
and therefore the reation artifacts are
00:30:26
much uh less over
00:30:29
here all right so I was talking about
00:30:32
the correction factor now this is used
00:30:35
when your biometer doesn't have a pseudo
00:30:37
fix setting or just has a pmma setting
00:30:40
now in those cases what you can do is
00:30:42
you can actually U put the mode as a
00:30:45
fake mode okay and then you can
00:30:48
calculate your axile length using the
00:30:50
ultrason biometer and after you have
00:30:53
calculated the axile length you can
00:30:54
actually add up the correction factor
00:30:57
for example if your patient has a pmma
00:30:59
intraocular lens inside the eye you will
00:31:02
carry out the biometry in the earth fic
00:31:04
mode and the Axel length say comes as 23
00:31:08
mm now in this person the correction
00:31:11
factor is plus 0.4 mm and therefore the
00:31:15
corrected axle length in this patient
00:31:17
would be 23 + 0.4 that is
00:31:21
23.4 MM okay similarly you can carry out
00:31:24
the correction factors for silicon and
00:31:26
also for the ACR
00:31:28
now let me tell you that if you already
00:31:30
have the settings for silicon and
00:31:32
acrylic iel then you don't need to take
00:31:35
these correction factor into
00:31:37
consideration all right now sometimes
00:31:40
there might be a patient who might be
00:31:42
having a silicone oil inside the eye now
00:31:45
silicon oil also can change the sound
00:31:47
velocity right it's it has high density
00:31:50
and uh for example we have 5,000 C
00:31:53
Strokes of silicon oil available in
00:31:55
which the velocity of the sound is going
00:31:57
to be 1 40 m/s and then we have a th000
00:32:01
c Scopes where the speed of sound is
00:32:04
about 980 m/ Second right as you can see
00:32:07
the sound waves are traveling slower in
00:32:11
the Silicon oil compared to the normal
00:32:13
eye and therefore if you don't really
00:32:15
use proper settings within your biometer
00:32:19
the the axi length that the biometer is
00:32:22
going to measure would be erroneously
00:32:24
long axial length all right so that's
00:32:27
one important point that you must
00:32:28
remember that silicon filled Globe is
00:32:31
going to lead to a false long axle
00:32:33
length measurement now to talk about
00:32:36
some common errors and challenging
00:32:38
situation while you're carrying out an
00:32:40
ultrasound biometry first thing first
00:32:43
whenever the inter eye difference is
00:32:45
greater than3 mm and when the
00:32:48
consecutive same eye readings are
00:32:51
different by more than 0.1 mm then in
00:32:54
those patients you have to be suspicious
00:32:57
the first first thing that you should do
00:32:58
is you have to cons uh consider the
00:33:00
medical history of the patient and find
00:33:03
out if there is any particular reason as
00:33:05
to why there are differences in the
00:33:07
reading the patient might be having a
00:33:09
macular pathology the patient might also
00:33:11
be having some problem like posterior
00:33:13
stoma which is going to give different
00:33:16
readings within the same eye all right
00:33:20
another common source of error which is
00:33:22
also the most common error seen in
00:33:24
contact technique is a corial
00:33:26
compression Okay so remember cornal
00:33:28
compression is seen in the contact
00:33:29
technique of biometry now this happens
00:33:32
because the eye is really soft and
00:33:34
pliable and the Cora can be indented
00:33:36
with minimal pressure also from the
00:33:38
probe tip and as a matter of fact the
00:33:40
softer the eye the lesser the
00:33:42
intraocular pressure and the greater is
00:33:44
the compression uh it's more easy to
00:33:46
compress a softer eye compared to a hard
00:33:49
eye and this will lead to uh the
00:33:52
problems within the axle length
00:33:54
measurement now since corneal
00:33:56
compression is going to compress in the
00:33:58
cornea the anterior chamber depth
00:34:00
measurement is also going to go down and
00:34:02
therefore in these cases it's very
00:34:04
important to keep an eye on the anterior
00:34:06
chamber depth if the depth is less you
00:34:09
know that there is some sort of cornal
00:34:10
compression which is going on and
00:34:12
therefore anterior chamber depth must
00:34:14
always be monitored and all the readings
00:34:16
with a shallow anterior chamber depth
00:34:18
must be deleted from your uh
00:34:23
measurements next uh error is the
00:34:25
misalignment of the probe I already told
00:34:28
you that it's very important to keep the
00:34:30
probe perpendicular to the coral vertex
00:34:33
and the Rays have to go and strike
00:34:35
perpendicularly to the macular surface
00:34:37
okay so that the rays are directed
00:34:40
parall to the visual axis this
00:34:42
perpendicularity is achieved whenever
00:34:44
this perpendicularity is achieved the
00:34:46
retinal Spike and the scar spikes will
00:34:49
be of high amplitude and the retinal
00:34:51
Spike will arise steeply from the
00:34:53
Baseline make sure that there are no
00:34:55
slopes no Jags no humps or steps on the
00:34:57
Ral spikes over here you can see that
00:34:59
this Ral spike is slightly sloping and
00:35:03
therefore this indicates that your
00:35:04
alignment of the probe is not correct
00:35:06
there's some misalignment so you need to
00:35:08
take another reading by proper placement
00:35:11
of the uh probe now sometimes the probe
00:35:15
the probe might be misaligned at the
00:35:17
lens surface okay so normally you have
00:35:19
the anterior lens Spike and the
00:35:21
posterior lens Spike so over here you
00:35:23
can see this is the anterior lens Spike
00:35:27
and this one over here is a posterior
00:35:28
lens Spike normally they should be of
00:35:30
equal amplitude if they are not of equal
00:35:33
amplitude it means that again the Rays
00:35:36
uh the sound waves are not uh striking
00:35:39
the lens appropriately that means there
00:35:40
is some sort of probe misalignment and
00:35:43
therefore you need to correct your
00:35:45
positioning now sometimes the probe can
00:35:47
be misaligned in such a way that the
00:35:49
Rays or the sound waves are going to
00:35:51
travel in uh through the optic nerve
00:35:54
instead of being instead of traveling to
00:35:56
the center of the maula right now in
00:35:59
such a case what is going to happen is
00:36:01
that there will be absence of the Scaris
00:36:02
spite now why does that occur we know
00:36:05
that the optic nerve basically is
00:36:07
actually a bundle of nerve fibers and
00:36:09
there's no Scara present within the
00:36:11
optic nerve and when the sound waves are
00:36:13
going to travel through the optic nerve
00:36:14
they're not going to encounter any
00:36:16
Scaris Spike now we don't want that we
00:36:18
basically are measuring the axal length
00:36:21
which is from the coral vertex up to the
00:36:23
internal limiting membrane in case of
00:36:25
ultrasound biom biometry and in case of
00:36:28
optical biometer we are measuring it
00:36:30
from the coral vertex up to the RP so
00:36:33
all these measurements are taken at the
00:36:34
macula right and therefore whenever you
00:36:37
see a waveform like this where the scar
00:36:39
spike is absent in those cases you
00:36:42
should know that there is misalignment
00:36:44
along the optic nerve all right another
00:36:48
thing is that make sure that there's no
00:36:50
uh big uh no thick gel sitting on the
00:36:52
patient's eye because then there's going
00:36:54
to be a miniscus between the probe tip
00:36:56
and the eye and you are going to get a
00:36:58
falsely long axial
00:37:00
length now another problem that occurs
00:37:03
uh while measuring the axial length is
00:37:05
extremely variable readings that you get
00:37:07
in case of posterior stomatis patients
00:37:10
and in high myopes now in high myopes
00:37:12
the globe is elongated and the uvia can
00:37:15
actually bulge into the Scara and this
00:37:17
happens mostly posteriorly now in these
00:37:20
cases the maula has a sloping Edge and
00:37:24
as I told you that the regularity and
00:37:26
smoothness of the interface is very
00:37:28
important in order to get good waves now
00:37:31
over here because there's a slope
00:37:33
configuration of the maula there will be
00:37:35
variable reflection of the sound waves
00:37:37
and therefore the waves that you see
00:37:39
over here would be of poor amplitude
00:37:41
there will be poor configuration
00:37:43
morphology and extremely variable
00:37:45
readings it's always better to carry out
00:37:48
an optical biometer biometry in case of
00:37:51
posterior stomas patient however if that
00:37:54
is not available you can carry out an
00:37:56
axi length measurement in a b scan as
00:37:58
well so in a b scan you do a horizontal
00:38:01
macular scan with the probe Mark present
00:38:04
um directed nely and the axle length
00:38:08
will be measured from the coral vertex
00:38:10
up to the maula over here what you see
00:38:12
is the optic nerve void so you take a
00:38:15
reading 4.5 mm below the optic nerve
00:38:18
void and this is how you can get the
00:38:20
axile length measure measurement in a
00:38:22
case of posterior stfy Lomas now we have
00:38:25
videos on B scan uh
00:38:28
B scan ultrasound as well on our channel
00:38:31
the link is going to be provided in the
00:38:33
description box now let us talk about
00:38:35
some of the advantages of an immersion
00:38:37
scan over the contact scan so here it is
00:38:41
more accurate than a contact scan
00:38:43
because the coral compression is
00:38:45
something which is avoided moreover you
00:38:47
will note that the immersion method
00:38:50
axile length are about 0.1 to 0.3 mm
00:38:53
longer than the contact method because
00:38:55
of course the uh the compression of the
00:38:57
cornea is avoided moreover the probe and
00:39:01
the corneal spikes are separate so you
00:39:02
can study the corneal spikes work the
00:39:04
cornea has two spikes over here okay
00:39:08
that is one from the endothelium one
00:39:09
from the epithelium it's a faster method
00:39:12
and moreover it reduces the technician
00:39:14
dependency now it doesn't mean that the
00:39:17
contact biometer is useless actually
00:39:21
speaking in the in good hands it
00:39:23
actually can give you really good values
00:39:25
and really comparable values but when
00:39:27
the technician dependency when the
00:39:29
technician is not as experienced and
00:39:31
therefore in those cases immersion scan
00:39:33
and an optical biometer is much better
00:39:37
choice all right so that's all for today
00:39:39
I hope you enjoyed the video if you did
00:39:42
don't forget to subscribe to our Channel
00:39:44
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00:39:46
all thank you and have a nice day