Training LabRAM Spectometer and Software

HORIBA Jobin Yvon
Training LabRAM Spectrometer and LABSPEC Software
Gwnalle Le Bourdon HORIBA Jobin Yvon SAS
Ref: Doc.TM-LabLS/En
The LabRAM Description, functioning and optical adjustment P.2

1. Description of the Spectrometer different parts and optical path
2. Alignment : frequency calibration, verification of the laser alignement,
change of the exciting wavelength
- LABRAM TRAINING
3. Optimisation of the options available: choice of grating, choice of

objective, slit and confocal hole
LabSpec how to obtain and save spectra P.34

1. Acquisition modes
2. Multi-point analysis
3. Raman mapping
4. Kinetics measurements
5. Depth profiling
6. Configuration menu (acquiqition parameters storage)
7. Saving options : formats, autosave mode
LabSpec Modes of visualisation and treatment of spectres

1. Visualisation options (spectra, mappings, depth profiles)
2. Spectra treatments : baseline, smoothing, peak fitting, normalisation
3. Mapping treatment
4. Modelling
Use with samples
1
- LABRAM TRAINING
1st PART
The LabRAM
Description of the spectrometer

Adjustments and optical alignment
2
- LABRAM TRAINING
LabRAM Description:
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4
The different parts of the LabRAM :
Laser :
- internal : HeNe 17mW. Wave length: 632,817 nm
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- external
Notch Filter :
1 Notch FIlter for each exciting wave length
Density Filters : To decrease the laser power

I = I0 x 10-D
By clicking her e, select one of the 6 neutral filters

with the optical densities 0.3, 0.6, 1, 2, 3 or 4.
filter [---] = no attenuation (P0 ), [D0.3] = P0 /2, [D0.6]
= P 0 /4, [D1] = P 0 /10, [D2] = P 0 /100, [D3] = P 0 /1000
and [D4] = P0 /10000
Microscope :
Illumination : 2 modes : transmission and reflection
Objectives : X10, X50, X100 (standard)
Confocal Hole: linked to spatial resolution
Close the confocal hole aperture
Initialize the confocal hole by closing

the hole and opening it to the previous
value.
Set the value of the confocal

hole aperture
Set the confocal hole to the maximum

value of aperture.
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5
Slit entrance : linked to spectral resolution
Spectrometer :
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2 gratings
Movement controlled by Sin Bar
Detector : CCD
5
6
Optical chamber :
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Upper part
of LabRAM
Spectrograph
Lower part of
LabRAM
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7
Optical Path and stem options:
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3
4
STEM
ACTION
ROLE
POSITION
Moves the beam

splitters BS12
Allows to choose
between a Raman
recording or a
visualization of the
laser sample
Pushed : visualization
with the camera
Pulled: Raman
measurement
Moves the block :

Allows to choose
Pushed : point mode
between
line
mode
Lenses L3, L4, L5, L6
Pulled: line mode
and
point
mode
and hole H2
Moves the mirror

M10
Moves the two

Choice between the
gratings 1800 g/mm two gratings
and 600 or 300
g/mm
Allows to choose
between the analysis
of a signal from the
microscope or from
the fiber optics
entrance
Pushed : point or
line mode
Pulled: fiber optics
analysis
Pushed : 1800 g/mm

grating
Pulled: 600 or 300
g/mm grating
7
Laser Alignment
This should be carried out when there is a significant loss of signal (a test to verify the
confocality by using a silicon sample will reveal any misalignment see P. 29-30) or when
the spot laser shows problems with the centering or focus.
- LABRAM TRAINING
Aim : to ensure that the laser is perfectly centred on the confocal hole image.
In order to do this, use the internal diode which follows the return path of the Raman
beam.
With the Labram, you have the possibility to see the image of the confocal hole
projected on the sample when you switch on the laser diode for alignment.
The laser diode for alignment is placed inside the spectrograph, and, when the
grating is turned at an appropriate angle, the diode beam exits from the
entrance slit of the spectrograph and illuminates the confocal hole. If you put a
flat reflective sample under the microscope (like silicon or even a glass surface)
you can see the projection of the confocal hole on it.
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9
Aligning the laser on the internal diode:
- LABRAM TRAINING
1. Turn on the internal diode:
2. Select the grating 1800 g/mm
3. Move the grating to the diode reference position
4. Position the camera for visualisation
5. Using the 100X objective focus on the silicon sample
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10
6. To locate the centre of the confocal hole easily, close to 100 m.
8. The diode spot determines the point which is used to align the spot laser.
There are two possible types of misalignment :
- LABRAM TRAINING
A centring problem:
A focusing problem:
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Should there be a significant disalignment of the laser, it is necessary to adjust the path by
using the mirrors as follows:
<Reference Laser 633nm>
You can adjust intensity by this mirror.
This mirror is very sensitive.
- LABRAM TRAINING
1,At first,you have to search maximum intensity by Z axis.

: Confirmation of intensity.
2,
3,Touch that mirror,and search maximum intensity value.
4,When you took a good value,you should check laser focus
after.
5,When you got bad focus,you can adjust by this mirror.

6,When you adjusted this mirror,you should check intensity
again.
<Others wavelength Laser>

You can adjust intensity by this mirror.
This mirror is very sensitive.
1,At first,you have to search maximum intensity by Z axis.
2,
3,Touch that mirror,and search maximum intensity value.
4,When you took a good value,you should check laser focus
after.
5,When you got bad focus,you can adjust by this mirror.

6,When you adjusted this mirror,you should check intensity
again.
A new confocality test has to be realised after the alignment (see P 29-30).
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Verifying the calibration frequency : zero order position of the gratings
The easiest way to test if your Labram is perfectly calibrated in frequency is to run a
silicon sample. You should find the Si 1 line at 520.7 cm-1.
If not, the zero order position of the grating has to be checked.
- LABRAM TRAINING
The gratings are driven with a sinus

arm that is linear in wavelength. In
fact the formula for the dispersion of
a grating is given by:
= [2cos(0)sin()]/nN , where N
is the number of grating grooves/mm;
n is the order and the angles 0 and
are represented in the picture. As

[2cos(0)]/nN is a constant, is
proportional to sin().
The coefficient ZERO is the mechanical position used as a reference for a value of
0nm. This corresponds to a number of steps of the motor between the switch of the
mechanical reference and the position 0 nm.
At the angle =0, the zero order of the grating must be centered on the detector. If it
is not the case, a constant shift in all the spectrum is observed (and thus on the silicon
band).
A small shift of the zero order can be produced by temperature changes. A shift of 6
pixels each 10 degrees of temperature change should be considered as normal.
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Adjusting the zero coefficient of the grating :
This is to be carried out for each grating.
- LABRAM TRAINING
1. Select the grating to be calibrated. Move the grating to the zero order position by
clicking on:
2. Select the following values for the confocal hole and slit entrance :
Hole = 400m
Slit = 150 m
Remove all samples and turn on the reflecting white light.
Let the white light enter the spectrometer by putting the camera beamspiltter.
Change the units of measurement to nm.
3. Use the icon :
to save a spectre and change the acquisition time of the intensity of
the light to obtain a signal around several thousands of counts.
4. Press STOP.
Use the red cursor to determine the position of the band. It should be
at 0 nm, at about +/- 1 pixel.
5. If the band is not at 0 nm, open the calibration window, by clicking on:
Before changing anything, note the values ZERO et KOEFF.
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- LABRAM TRAINING
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In the second menu Mfluo , change the value of ZERO :
Zero value [+] : Spectrum is going to minus direction.

Zero value [-] : Spectrum is going to plus direction.
Now adjust the ZERO and watch the band position move, adjust until the band is within
+/- 1 pixel of 0 nm
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- LABRAM TRAINING
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6. Now change the UNITS to cm-1 and move the spectrograph to the position at which you
should monitor the Si Raman band (520.7cm-1) at the centre of the CCD (the central pixel
corresponds to the pixel for which one the frequency position is the same than the
spectrograph window value).
7. Insert your standard silicon sample and focus the laser in the normal way. Using the
spectrum adjustment icon
line. Press STOP.
again , you should now be able to see the Silicon Raman
8. Again use the RED cursor to measure the position of the band. It should within +/1pixel of 520.7cm-1.
9. Once you are satisfied with the calibration, close the calibration window and ensure that
you save the changes when prompted.
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Notch Filter
The Notch Filter is used to reject the laser and filter
- LABRAM TRAINING
the Rayleigh diffusion.
EASY
OPTICAL
DENSITY
7
6
POSSIBLE RAMAN
5
4
NO RAMAN
3
2
(degree)
0
15
10
T (%)
100
80
60
40
RAMAN
(cm-1)
20
0
0
50
100
150
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Characteristics of Notch Filters :
1 : filter references
2 : transmission of the filter
in function of the angle
3 : optical density in
function of the angle
4 : cut-off position in
5 : spectral edge width in
2
Edgewidth and cut-off definition

edgewidth
1
0
-1
-2
-500
4
4
5
5
80
Intensity (%)
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Wavenumber
(
1)
60
40
50 %
20
0
-500
0
Wavenumber (cm-1)
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Aligning the Notch Filter.
Notch filter
- LABRAM TRAINING
Spacer
Spacer Number
Diameter (mm)
Angle of the
notch (degrees)
1
4
9,84
2
5
8,69
3
6
7,58
4
7
6,59
5
8
5,69
6
9
4,86
7
10
4,05
8
11
3,3
NB. Each Notch Filter must be used with the adapted spacer.
You can see the position of the cut-off of the notch filter looking at the white lamp in
transmission with a x10 objective. If the spectrograph is positioned on the exciting line
you can record a spectrum like :
The cut-off of the

notch
is
often
asymmetrical,
to
achieve a lower edge
of transmission. The
lowest wave number
that can be measured
reliably is around
100-120 cm-1.
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Hardware Section
Practical Advise Sheet n1 : Changing the excitation wave length
1. Removable mirror
2. Changing the Notch Filter (remember to choose a suitable spacer)
- LABRAM TRAINING
3. Software : enter the new wavelength value.
4. Choose a suitable grating (see p.20)

5. Position the spectrometer in the centre of the spectral window.
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Hardware Section
Practical Advice Sheet N2 : Choosing a suitable grating
The spectral resolution depends on :

- the grating
- the slit entrance
- LABRAM TRAINING
- the excitation wavelength

- the spectometers focal distance
- the number of pixels of the CCD
Parameters which can be optimised by the user:

- the grating
- the excitation wavelength
- the size of the slit entrance (in most cases a slit of 100 m is used)
Depending on the grating selected:

- the resolution differs
- the observed spectral range will differ
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- LABRAM TRAINING
Influence of the grating :
Gratings at fixed positions (1700 cm-1)

10000
1800 l/mm
600 l/mm
Intensity (a.u.)
8000
6000
4000
2000
500
1000
1500
2000
2500
Wavenumber (cm-1)
21
707.9
22
12000
Different gratings same excitation wavelength

10000
953.7
939.4
966.1
923.5
908.8
4000
- LABRAM TRAINING
1800 l/mm
600 l/mm
929.9
6000
695.2
Intensity (a.u.)
8000
2000
700
750
800
850
900
950
1000
Wavenumber (cm-1)
To conclude:
Choice of grating depends on the application and aims of the measurement.
NB : other grating characteristics :

- The gratings are appropriate to a certain wavelength, meaning they have a reflection
maximum in certain spectral ranges.
The reflection of a grating is hence subject to the wavelength (1) and the light polarisation
(2)
TE light polarized parallel to the grooves
TM light polarized normal to the grooves
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IMPORTANT when working in the Near InfraRed!
- choice of grating (the grating 1800tr/mm is not suitable : optimised in visible and limited
mechanically)
950 tr/mm
- effect of the detectors response
Quantum efficiency, % .
60
633 - 787 nm
50
40
30
780 - 1030 nm
20
10
0
200
300
400
500
600
700
800
900
1000 1100
Wavelength, nm .
32000
30000
Pine excitation at 633 nm

Pine excitation at 780 nm
28000
26000
24000
22000
INT [a.u.]
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Typical spectral response at 193 K .
20000
18000
16000
14000
12000
10000
8000
6000
4000
2000
0
250
500
750
1000 1250 1500 1750 2000 2250 2500 2750 3000

-1
Wellenzahl [cm ]
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Hardware Section
Practical Advice Sheet n3 : choosing the best objective
Numeric aperture of an objective : N.A. = n. sin(m)
m being the half open aperture
and n the refraction indice
- LABRAM TRAINING
Maximum diameter of the luminated spot is
NA = n sin ()
limited by diffraction phenomenas:

T = 1,22 x ( / NA )
eg : for a x100 objective of NA: 0,9
T = 1,22 x ( 632,81 / 0,9 )= 858 nm or 0,86 m
This resolution can be limited by the confocal

hole.
Lateral Resolution
Optical characteristics of the main objectives used:
Type of objective
10
50 X
50 X
100 X
100 X
LWD
MPlan
LWD
MPlan
33.4
48.6
53.1
64.2
Half aperture
max (m)
NA=n.sin (m)
0.25
0.55
0.75
0.8
0.9
W. D. (mm)
8.1
0.38
3.2
0.21
Spot diameter
3.1
1.4
1.03
0.96
0.86
632.8 nm
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Axial resolution field depth
The depth probed depends on the numeric aperture (NA) of the objective :
B High aperture : small volume studied
B Low aperture : large volume studied
The choice of objective will determine the intensity of the Raman spectra. Depending on
the sample type (opaque or transparent), the same objective will not have the same
- LABRAM TRAINING
behaviour.
1 Opaque sample
When there is almost no penetration of the laser in the sample, the Raman spectrum is
obtained mainly from the surface and its intensity is proportional to the collected flux. It
will be better to use a microscope objective with a high numerical aperture (x100,
NA=0.9) so that the solid angle (NA = nsin()) is bigger and you have a maximum
Raman signal.
The following drawing compares a x100 objective with a macro objective, which supports
this argument.
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Silicon line intensity = f(NA)
100
obj 100x
90
80
Intensity (%)
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70
obj 50x
60
50
40
30
20
10
obj 10x
0
0
0,2
0,4
0,6
0,8
Numerical Aperture
2- Transparent sample
If you have an homogenous sample, it will be better to use a microscope objective with a
big depth of focus (for example a x 10) so that it will collect the signal from a bigger
volume with a macro objective supports this argument.
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Hardware Section
Practical Advice Sheet N3 : Confocality
The principle of confocality
- LABRAM TRAINING
Confocal Hole
Rejected
Beams
Multilayered sample
Advantages :
(1) small increase in the lateral resolution
(2) large improvement in the axial resolution
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Relationship between the aperture of the confocal hole (m) and the signal intensity (%)
- LABRAM TRAINING
This is also a test to verify the laser alignment.
Relationship between Depth (m) and

Intensity (a.u.) For 6 Confocal Hole
Apertures from 100 to 1100 m
Relationship between Confocal Hole

Aperture (m) and Axial Resolution (m)
(Full Width at Half Maximum)
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Use of a quick confocality test to check laser alignment
Device
bar
- LABRAM TRAINING
Take a
spectrum
: Take in spectrum. (1 sec)
: Take in spectrum. (1 sec)
Device bar
Take a
spectrum
Check
Choose a 1000um spectrum.

: Select this icon.(Multiply Const)
Calculate the ratio of 1000um to 200um.
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Laser He-Ne (632.817 nm) :

-
The optimum confocality value = 60% with a confocal hole at 200 m/

confocal hole aperture at 100m
The laser is required to be adjusted if confocality becomes <40 %
Diode laser 785 nm :

-
Optimum confocality value = 35-40 % with a confocal hole at 200 m/

confocal hole aperture at 1000m
The laser is required to be adjusted if confocality becomes <20 %
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Harware Section
Practical Advice Sheet N4 : Taking measurements in Macro
- LABRAM TRAINING
With the Labram you have the possibility of working with macro-samples, gases and
liquids. For that you have to mount the accessory that is shown in the drawing below
which replaces one of the microscope objectives.
This macro-sampling device uses a 40 mm focal length lens, but other focal lengths are
available. You can even mount a microscope objective at the place of the 40 mm lens.
The advantage is that your laser beam exits horizontally and not vertically. An accessory
with a spherical mirror for double laser pass is also available for transparent material (see
below).
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Troubleshooting : I cant acquire my spectrum
- LABRAM TRAINING
Check the following :

- Wavelength (nm/cm-1)
- Camera pull handle
- Z axis (Focus)
- Try reinitialization. (Hole/Slit/Wavelength)
- Is there some obstacle on light axis? (Paper)
- Checking of Power supply switches.
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Troubleshooting : My spectrum look odd
- LABRAM TRAINING
Check :
That the internal diode hasnt been left on
That the white light is switched off
That the light in the room is switched off
Troubleshooting : My spectrum have a weak intensity
Check :
That there is no density filter on the laser beam
That the objective is clean
If necessary, clean the obhective with a mix 5% ether / alcohol. Soak the lens and place it
in an ultra sound bath.
Aligning the laser on a silicon sample (check the spot is centred and there is no
major focusing problems)
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- LABRAM TRAINING
Second Part
LabSpec
Acquiring and saving a spectrum
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5 Practical Advice Sheets for acquiring :

- a spectrum in point mode
- spectra at multiple points in the sample
- a Raman mapping
- kinetics
- LABRAM TRAINING
- an in-depth profile
Precautions before recording spectrum :

Be sure that the laser power will not harm the sample ! Use density filters to decrease the
laser power in case the sample is sensitive to laser heating.
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Practical Advice Sheet N1 : recording a spectrum / point mode

1. Choosing the grating
Select the grating from the LabSpec software (LabRAM : a message will appear asking to
- LABRAM TRAINING
choose the correct stem position for the grating)

Click here to select one of the available spectrograph gratings
Do not forget to initialize the spectrograph after a grating change
Choose the grating with the use of stem 4.
In case the grating has not been used before, check its zero order.
Move the spectrograph to the
zero order position (0 nm)
2. Focusing the laser

Using either the video monitor or the video image function within LabSpec
3. Positioning the spectrograph

Centre the grating at the desired position
Enter here the spectrograph

position value
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4. Define the size of the slit (100m) and that of the confocal hole
5. Define the parameters exposure time and number of accumulations
Number of accumulations
- LABRAM TRAINING
Exposure time in seconds
3 possible acquisition modes
Type of acquisition
Simple window
Adjustment
Multi-window
Accumulation Mode
Parameters to define
Note
- Acquisition time
The previous
- Central position of the spectral
spectrum is
zone
automatically erased
- Acquisition mode
- Number of accumulations
- Complete spectral mode
(Multi-window)
Scanning Mode
Continuous (Kiefer
Scanning mode)
- Acquisition time
- Kiefer Scan parameters
(Spectral zone and number of
accumulations)
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Principle of the different acquisition modes :
Generally to get the whole Raman spectrum, multiple spectral windows are required. This
is achieved by moving the grating position in the spectrometer in some manner so as to
move the specific part of the spectral range which illuminates the CCD.
The first option is to use discreet spectral windows, which are glued automatically. (see
multi window acquisition option).
60000
50000
Intensity (a.u.)
- LABRAM TRAINING
Multi-Window Mode
40000
30000
20000
10000
0
500
1000
1500
2000
2500
3000
3500
Wavenumber (cm-1)
Kiefer Scan Mode

The method used by the new Kiefer scanning works in a different way and consists of
shifting the spectrum step by step so that each individual spectral element is detected
several times by the detector, rather than as a discreet spectral window.
The software and hardware can scan the spectrometer through a defined spectral region,
off-setting each subsequent acquisition viewed by the CCD detector to a certain amount.
This can be by a large number of pixel steps or even a sub-pixel value, depending upon the
required effect.
(i) Mode (I) - Larger Pixel overlap values :
In mode (I), a larger number of pixels is chosen as the offset, and an averaging effect is
produced. For this method the operational principle is that a datapoint ( in cm-1 ) is seen by
a number of different pixels on the CCD detector, and the average signal for this datapoint
is calculated.
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3000
Intensity (a.u.)
2500
2000
1500
500
500
1000
1500
2000
Wavenumber (cm-1)
(i) Mode (II) - Sub pixel offset.

The second way of using the Kiefer CREST scan is to use very small overlaps in the
spectrum, which provides an enhanced band definition.
Here a shift in position, entered in the sub Pixel value box, will move the grating
position by an amount less than one pixel on the detector. - A Sub Pixel.
By selecting a sub-pixel value (a value of 1 is for full integer values and hence
deactivates this mode), the step selected will increase the number of data points
obtained for the spectrum. Hence, a 2 subpixel value will give twice the number of
data points, 3 subpixel value three times and so on.
If you consider a usual acquisition, you have 1024 pixels (and 1024 data points).
Using the subpixel arrangement of a factor of 2, will give 2048 data points.
Whilst this operation does not affect the actual spectral resolution which remains
defined by the spectrometer focal length, grating and entrance slit, it does provide a
better band definition for Raman bands and can hence provide a better basis for
analysis of band shape and position for a given instrument.
8000
Intensity (a.u.)
- LABRAM TRAINING
1000
6000
4000
2000
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0
428
430
432
434
436
438
Wavenumber (cm-1)
40
How to use the Kiefer Scanning Modes?
- LABRAM TRAINING
indicates the Kiefer scanning modes, by clicking on this, the window for the
Kiefer Scan will open:
start point is the starting point for the spectrum you wish to have (in cm-1 or in
nm)
finish point is the end point for the spectrum you wish to have (in cm-1 or nm)
accumulation number activates the first mode of the Kiefer scan used to
generate extended spectral regions and for spectral averaging, Mode (I)
The value represents how often a spectral data element will be detected (any value
can be entered) ie. the larger the number the greater the averaging.
sub-pixel factor defines the linearized data point (maximum is 6).
This is used to generate the higher definition mode. Again the greater the value, the
greater the definition, Mode(ii).
It can be considered that there are three cases for using the Kiefer scanning:
reduction of spectroscopic phenomenon ( on a wide spectral domain):
1) just enter the start point and finish point values,

2) select the accumulation number required
3) and set sub-pixel factor to 1.
4) Press start and the software drives the spectrograph, acquires the data and
linearizes the spectrum.
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The selection of the accumulation number depends on the required quality of the
end spectrum. The higher the number, the better the quality.
Integration time : for instance, if integration time T for classic acquisition is selected
and N accumulation for the Kiefer Scanning is also selected, the integration time
should be changed to T/N before starting the Kiefer Scanning.
- LABRAM TRAINING
- Improving the definition of the line shape ( on a short spectral domain) :

1) just enter the start point and finish point values,
2) set the accumulation number to 1
3) and select the sub-pixel factor required
4) Press start.
For the same reason as above, change the integration time to a lower value.
- A combination of both modes is possible but this is not really recommended as

this method will take time, especially if you require a complete Raman spectrum
with a definition four times better!
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Practical Advice Sheet N2 : recording spectra in several points in the

sample (Multi-points analysis)
- LABRAM TRAINING
LabRAM equipped with a motorised XY table
1.
Focusing the laser on the sample
2.
Recording the video image on the sample surface

Stop the acquisition of the continuous video
3. Define the measurement points with the cursor
4. Define the acquisition parameters :

- grating
- acquisition time and number of accumulations
- spectral zone multi-window
- confocal hole aperture and slit entrance
5. To start an acquisition use the icon spectral image
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Practical Advice Sheet N3 : recording Raman Maps

LabRAM equipped with a motorised XY stage
Initially, determine the best measurement conditions (acquisition time and number of
accumulations, confocal hole and slit apertures, density filter, spectral range) by
- LABRAM TRAINING
acquiring some few spectra in different areas of the sample. This allows one to optimize
the parameters and to prevent from detector saturation.
1. Displaying the sample with white light

Verify that the objective selected in LabSpec corresponds to the objective used.
Recording the video image
2. Open the window Acquisition Options
Select table in the sub-menu X-scanning and Cursor in scanning area.

Define the value in Refresh Time :which determines the period of time between the
two updates displaying the spectrum recorded on screen. In case of a long mapping
increase this time (eg. 3600 s) in order not to lose time with the use of display updates.
Close the Acquisition Options window.
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3. Choosing the cursor type to define the zone analysed
- a-
sloping line
- b-
horizontal line
- c-
rectangle
- d-
elipse
- e-
polygon
- LABRAM TRAINING
3. Selecting the parameters of the measuring zone

Open the Acquisition Data Parameters window
- Click on X and Y to define either the number of measurement points or the steps
between two points (m), then the software calculates automatically the second
parameters.
4. Define the acquisition parameters:

- grating
- acquisition time and number of acquisitions
- multi-window spectral zone
- Apertures of confocal hole and slit entrance
5. To start an acquisition, use the icon spectral image
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Practical Advice Sheet N4 : recording Kinetics
This option enables you to take a series of spectra or spectral images as a function of time.
Follow the same procedure as the one to record point by point spectra or spectral images.
- LABRAM TRAINING
But you also have to choose:
In the Data size window (select the time parameter, there are two types of boxes, the
first is the number of measurements and the second is the time interval between them).
Please refer to the Index section
Be careful, because the acquisition time is included in the interval of time between two
measurements.
To start an acquisition, use the icon spectral image
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Practical Advice Sheet N5 : Recording a profile in depth
Focus the laser on the sample,

Take a video image and freeze it with the icon,
- LABRAM TRAINING
Choose the cursor,

Select the time of exposure,
Select the
In the window Data size , select the Z scanning parameters.
- Please refer to the Index section
Press the icon
to start the acquisition
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47
Saving the measuring options
- LABRAM TRAINING
Configuration Window
47
48
Saving spectrum
Save one of the displayed spectra, by activating the spectrum window, select the
desired spectrum by pressing the radio button, then choose one of the following
methods:
- LABRAM TRAINING
Click on the following icon:

then enter the file name, its location and format.
From the file Main Menu, select the Save As option, then enter the file name, its
location and format.
Before saving, it would be useful to complete the information list about the spectrum
(operator, laser power, etc...) by pressing the icon
NB. Some parameters (hole, slit, spectro, grating, time, accum, date) are automatically
updated.
LabSpec file formats.
The following is a list of the various file formats that LabSpec supports to save the
acquired spectra or images:
Dilor ASCII format (*. ms0): This format is used for single spectrum.
Extended Tiff
- (*.tsf):
It is a specific format for single spectrum and
LabSpec software.
- (*.tvf):
It is a specific format for spectral image.
Standard Tiff (*.tiff): Standard TIFF format for image.
Text format (*.txt): This is an ASCII mode format which uses two columns:
wavelength/Wavenumber and intensity, without header.
Spectra Calc format (*.spc):
processing softwares.
This format is used by SpectraCalc and Grams
Important comments:
- It is possible to save several spectra one after the other by using MULTI, (do not forget
to de-select after use) icon:
- when saving as txt, remember to activate Axe+Text
- Saving images:
The save procedure always saves the content of the active window. To save an image,
activate the window that contains all the spectra. If the Spectrum: Point window is
activated, only this spectrum will be saved, and not the whole spectral image.
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49
Saving in ASCII Format
- LABRAM TRAINING
This module permits to save all the spectra (or the spectra of a Raman image) of a window
as ASCII files (the maximum spectra saved in one shot is 64)
Destination path : indicate the address of the directory where the spectra will be saved.
Conversion option :
Different conversion options are available:
to remove the converted objects of the LabSpec window.,
to split the activated image to spectra that will be saved in ASCII
format,
to saved the ASCII file in two columns or two lines
to write the frequency values and/or the position values.
To activate the saving of the spectra press the button : SAVE ALL
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- LABRAM TRAINING
Auto Save
- You can choose the directory where the spectra will be recorded:
Yo u can choose a name
You can choose to use

the day, the month and the year as the name
MAXIMUM 8 CHARACTERS
- You can choose the file name of the recorded spectra:
Yo u can choose a name
You can choose to increment

the name by number, hour and minutes
of the acquisition.
MAXIMUM 8 CHARACTERS.
- You can choose the format of the files:
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Two options are available:
You can choose to work with the Auto Save and Auto Repeat options:
For this the delay between two acquisitions (eg: 10 seconds) must be chosen. Then after
clicking on the
icon the software takes an acquisition and repeats every 10
seconds, saving the spectra automatically.
- LABRAM TRAINING
However it is possible to work only with the Auto Save option:

- When the icon
it.
is selected, the software takes an acquisition, stops and records
- When the icon

is selected (which is used for spectral imaging, time scanning...)
the software takes a spectral image and at the end of the acquisition will be recorded.
MAKE SURE TO CHOOSE THE TSF FORMAT FOR THE SPECTRAL
IMAGES.
51
- LABRAM TRAINING
52
Third Part
LabSpec
Processing Spectra and Raman Mappings
52
53
Baseline Correction
Automatic
calculation
- LABRAM TRAINING
Additional/Subtraction
Clears the points
of the baseline
Saves as a
spectrum
To save the
baseline
Normalise the
spectrum
(maps)
The main procedure is to build up a baseline point by point, to best fit the spectrum and
then subtract it from the spectrum.
If you have to subtract the baseline from a spectrum, activate this spectrum.
If you have to subtract the baseline an image, activate the spectral image window.
Verify that the option Ins/Del is active (in the operations box)
Select the type for interpolation: it can be linear or polynomial (in the box type). For
the polynomial interpolation, you can also choose the degree of the polynom (in the
degree box).
You can select with the mouse in the spectrum window (validate: left button, delete:
right button) the points for the baseline computation
Hint:
(for the images, when you press the icon
average spectrum of the image is opened automatically).
, a window that contains an
Activate the option attachment , to fit at best the baseline to the spectrum.
Hint:
An automatic procedure can also be used for the computation of baseline:
button Auto
Press the button SUB .
NB: The baseline can be saved as a spectrum: by selecting the CONV button
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Correction
- LABRAM TRAINING
Main use for processing images:

Enter the weakest value for the spectra as 0 and normalisation.
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Profile
2 main usess :
- LABRAM TRAINING
- (1) to create a profile file with several spectra separately saved and required to be
treated as images
- (2) to extract the profiles from a map.
(1) Create an image with several spectra : use the Add function after having activated the
spectrum into which the profile is to be added.
(2) Extract a profile from a map, either by following the horizontal or vertical lines.
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- LABRAM TRAINING
Peak-fitting
Preparation : Remove spikes on the spectrum

NB: in the case of an image, this modification must be carried out for each spectrum. If a
spectrum has a spike, remove this spike in the window Spectrum : Point and Press
button R to insert the corrected spectrum in the Raman mapping.
Step 1 : If only one part of the spectrum is of interest, first extract this zone by using the
window:
(if it is a spectrum or image)
Then, define the approximative positions of the bands

- by an Auto search (height parameter and neighbour to adjust)
- by using the following icon
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- LABRAM TRAINING
Step 2 : define the function for fitting/add a baseline
It is possible to choose a function independently for each band.
Step 3 : Define the parameters: number of iterations and deviations

Then start the peak fitting operation by clicking on
Then on
Step 4 : Visualise the reults by activating Band sum and Band shape.
Then for a table click on
57
- LABRAM TRAINING
58
p : frequency position of the band.

a : amplitude of the band.
w : width at half maximum.
s : surface of the band.
g : Gaussian/Lorentzian ratio.
NB : it is possible to save these results by using the SAVE function
NB. : it is possible to fix the value of a parameter
Step 5 : with images

It is possible to draw up a map for each of the predetermined parameters by pressing keys
p , a , w , g or s .
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Examples of Raman mapping based on band Intensity/Frequency/Width (Thanks to Mr
Mermoux) :
- LABRAM TRAINING
Length Y (m)
200
300
x1000
400
50
500
intensit
600
400
500
600
Length X (m)
15000
1333.0
1333.0
1332.8
1332.8
1332.6
1332.6
frquence
10000
2.4
5000
2.2
Images : 4500 pixels

(pas de 5 m)
2h30 acquisition time
0
1200
largeur
1400
Backg
intensity
x1000
200
150
40
100
10 m
20
50
TEM
1340
10
1335
5
1330
frequency
width
100 microscope objective
Cathodoluminescence
Point spacing: 0.7 m

exc.=514.5 nm
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Modelling
It is the decomposition of each original spectrum of an image as a sum of model
spectra.
Choose the spectra that will become MODELS , which can be already saved on the
- LABRAM TRAINING
disk, or they can be particular spectra that have been extracted and saved from a spectral
image.
If the spectrum is a particular and extracted from the image and save.
Do the same with any other interesting spectra.
Load all the selected spectra and put them overlapped in a window (for that use the
option Behavior in the menu view in the FORMAT menu).
Activate the first spectrum selected and press the button get. Do the same for all the
selected spectra: a window is then created with all the model spectra .
In the single spectrum window, there are:
- The models with relative intensity.

- The experimental spectrum in particular point of the image.
- The result of the fitting.
You will see in the mapping window additional pictures that correspond to each one of the
model .
You can overlap them to see the relative contribution of each of the spectra in a particular
point of the image (for that use the option Behavior in the menu view in the
FORMAT menu
You can save a whole spectral image with the model compounds choosing the tvf
format. When loading this image, the decomposition will automatically appear.
60

Training LabRAM Spectometer and Software

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HORIBA Jobin Yvon

Training LabRAM Spectrometer and LABSPEC Software

Gwnalle Le Bourdon HORIBA Jobin Yvon SAS

The LabRAM Description, functioning and optical adjustment P.2

3. Optimisation of the options available: choice of grating, choice of

LabSpec how to obtain and save spectra P.34

LabSpec Modes of visualisation and treatment of spectres

Use with samples

Description of the spectrometer

Density Filters : To decrease the laser power

By clicking her e, select one of the 6 neutral filters

Confocal Hole: linked to spatial resolution

Close the confocal hole aperture

Initialize the confocal hole by closing

Set the value of the confocal

Set the confocal hole to the maximum

Moves the beam

Moves the block :

Moves the mirror

Moves the two

Pushed : 1800 g/mm

1. Turn on the internal diode:

2. Select the grating 1800 g/mm

3. Move the grating to the diode reference position

4. Position the camera for visualisation

5. Using the 100X objective focus on the silicon sample

6. To locate the centre of the confocal hole easily, close to 100 m.

There are two possible types of misalignment :

1,At first,you have to search maximum intensity by Z axis.

5,When you got bad focus,you can adjust by this mirror.

<Others wavelength Laser>

5,When you got bad focus,you can adjust by this mirror.

Verifying the calibration frequency : zero order position of the gratings

The gratings are driven with a sinus

are represented in the picture. As

In the second menu Mfluo , change the value of ZERO :

Zero value [+] : Spectrum is going to minus direction.

again , you should now be able to see the Silicon Raman

the Rayleigh diffusion.

Edgewidth and cut-off definition

The cut-off of the

3. Software : enter the new wavelength value.

4. Choose a suitable grating (see p.20)

The spectral resolution depends on :

- the excitation wavelength

Parameters which can be optimised by the user:

Depending on the grating selected:

Influence of the grating :

Gratings at fixed positions (1700 cm-1)

Different gratings same excitation wavelength

NB : other grating characteristics :

- effect of the detectors response

Pine excitation at 633 nm

Typical spectral response at 193 K .

1000 1250 1500 1750 2000 2250 2500 2750 3000

Maximum diameter of the luminated spot is

limited by diffraction phenomenas:

eg : for a x100 objective of NA: 0,9

T = 1,22 x ( 632,81 / 0,9 )= 858 nm or 0,86 m

This resolution can be limited by the confocal

Silicon line intensity = f(NA)

The principle of confocality

This is also a test to verify the laser alignment.