CMi SOP003 Operating Procedures Manual - User Manual

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CMI | SOP003_rev1.0

CMI STANDARD OPERATING PROCEDURE

Confocal Raman Microscope

Physiology Ground floor research lab

CMI document ID: SOP003

CONTACT INFORMATION:

Peter Owens: 091 494036 (office)

Peter.owens@nuigalway.ie

Jennifer Connolly: Jennifer.connolly@nuigalway.ie

REQUIREMENTS FOR EQUIPMENT USAGE:

1. CMI user

2. Completion and signing of Microscope Safety Checklist

3. Certification by Peter Owens or Jennifer Connolly

REVISION LOG

Revision

Date

Author

Changes

1.0

12/5/14

P. Owens

Initial draft

Purpose

1.1.

This document specifies the work instructions for the CMI Witec Confocal Raman microscope located in

the ground floor Physiology lab, Quadrangle building. If you see an area where more clarification is

needed, if additional information is needed, or if you have suggestions on how to make this guide more

useful in the lab, please contact the CMI.

1.2.

Note that this document is not a detailed instrument manual and does not intend to be one. For

detailed questions or if anything unusual happens with the system, please refer to the manuals

present in the lab, or ask CMI personnel for help.

CMI | SOP003_rev1.0

Scope

These work instructions are applicable to

all

work that is carried out using the Witec raman microscope.

Important notes

PLEASE LEAVE ALL HARDCOPIES IN THE LAB

3.1

Laser safety guidelines

The WITec microscopes uses

class 4

633 and 785 nm laser sources during operation. The

safe use of lasers requires that all laser users, and everyone near the laser systems, are aware of the

dangers involved.

CAUTION: Direct eye contact with the output beam from a laser will cause serious damage and possibly

blindness.

The 785 nm laser has a high power output, extreme care is needed here when operating the

system.

3.1.1

Make sure the enclosure remains closed during laser scanning and measurement

3.1.2

Always close the laser shutter before opening the door of enclosure

3.1.3

Always wear the safety laser goggle when you want to open the door with laser on for

alignment procedure.

3.1.4

Participation in a Laser safety course is strongly recommended for operating this system.

3.2. Witec Alpha 500 manual (hardcopy in the lab, soft copy on the instrument PC), and training notes

3.3 The CMI access policy, available online at

http://imaging.nuigalway.ie/access%20policy/cmi_access_policy_1.6.pdf

3.4

This manual was developed to assist in the training process of users. Be aware that only the basic

operation details will be presented. Please contact the CMI staff for more assistance if required.

3.5

Changes may occur when a new software version or patch is installed. Please contact the CMI

staff if you are not sure about new features and functions.

3.6

Do not forget to sign in to the log book before you start your measurement.

3.7

Turn on the laser power when you begin, use laser shutter in-between measurements.

Responsibilities

Operators of this equipment are responsible for the following:

4.1

Complying with all safety regulations.

4.2

Compliance with procedures and specifications contained in this document.

4.3

Reporting misuse of the instruments, or in a manner inconsistent with this specification, by any

CMI | SOP003_rev1.0

personnel, to the supervising CMI staff.

4.4

Maintaining a clean workspace.

Food and drink are NOT allowed

4.5

Reporting any and all maintenance issues/concerns to the supervising CMI staff member

immediately.

Raman overview

Raman spectroscopy is a characterization technique that is widely used in scientific field in recent years. It

actually utilizes the unique Raman spectra for different components as a spectral “finger print” to identify

unknown samples or even further analysis based on the information from the spectra. Raman spectra can be

obtained from various kinds of materials from bulk solids such as paper and cellphone, to nanomaterials such

as thin films and nanoconstructs.

Raman Spectroscopy has many advantages among many characterization techniques, and therefore it is quite

welcome in scientists and laboratory workers. Typically, the samples need little preparation before

characterization and analysis can be carried out through many containers. Raman Spectroscopy is usually not

destructive to samples unless you use too much laser power and focus high-energy laser on a point of the

sample, leading great amount of heat in that small area and thus burning your sample.

In addition, Raman Spectroscopy is typically a fast characterization technique that can perform real-time scan.

It can acquire a Raman spectrum of most substances in seconds via Charge Coupled Device detectors (CCDs)

that have a wide dynamic range for users to select the appropriate exposure time for their sample. Depending

on the raman cross section of the sample of interest, a high resolution scan can be finished in minutes using

the system.

Raman Spectroscopy can do both qualitative and quantitative analysis. Quantitative analysis of the sample is

typically performed by measuring the relative intensities of each peak in the Raman spectrum that are directly

proportional to the relative concentrations of the compounds. Alternatively, chemometric methods can be

used for detailed information and accurate calculation. These quantitative analyses are very sensitive that can

be performed on samples with high concentrations ranging from 90-100% material of interest down to

concentration determination at parts per billion (PPB) levels.

This instruction will guide you to run a Raman spectroscopy scanning step by step and help you obtain your

first Raman spectrum/ image from the WITec Raman

Spectroscopy Instrument. It can also be used as a manual

book for laboratory users in case of operational problems and troubleshooting. This instruction is separated

into sections for instrument overview, step by step alignment and calibration check, acquisition, imaging, and

troubleshooting. Readers should follow the procedures in this instruction in order to operate the Raman

instrument properly.

DANGER: Class 4 laser radiation involved during the procedure!

CMI | SOP003_rev1.0

System Overview

The witec confocal raman microscope consists of the following devices:

6.1

Instrument Control PC, 64 bit running witec control and project software (version 1.6)

6.2

Controller unit.

6.3

Upright microscope with led light source for brightfield work.

6.4

Objectives including a 40x water dipping lens and 100 x air

6.5

Andor CCD cameras

6.6

Witec diffraction gratings for either vis or NIR operation.

6.7

Motorised stage for xyz control

6.8

Fibre optic cable for 633nm use: 50micron diameter

6.9

Fibre optic cable for 785 nm use : 100 micron diameter

Familiarise yourself with the system folders, located on the shelf above the equipment.

Start Up Procedure

7.1

Book equipment on CMI web booking system.

7.2

Turn on lasers or individual laser, if only one is to be used. For the 633 laser, turn on the key. For
the 785 nm laser, turn on power first and wait until the green led stops flashing. Then switch the
laser key to ‘on’ and again wait until the green led stops flashing and both yellow and green leds

Fibre to detection
system. Use 50 micron
fibre for 633 nm, 100
micron fibre for 785nm
excitation, fibre
diameter is part of the
serial number taped on
fibre.

Extreme care

needed when handling
flibre cables.!!!

Adjustment
screws for
alignment

Push/pull rod for
eyepiece/detector

Laser coupler
and filter wheel

Eye piece
camera

785nm laser

Brightfield/DIC/Ra
man imaging
selection

CMI | SOP003_rev1.0

are continuously on.

7.3

Turn on power to controller if not already on.

7.4

Turn on power to camera(s). Turn on only the one you are planning to use :

7.5

Turn on PC, login password is ‘biophotonics119’.

7.6

Both the lasers have to be warmed up for at least 30 mins before acquisition; while warming up
alignment of the microscope can be done.

7.7

Click on the ‘Witec Project Control’ to start the raman software interface

633nm laser

785 nm laser

Modulate
laser
intensity

Diffraction grating
for visible spectrum

Diffraction grating
for NIR spect

CCD camera VIS

CCD camera NIR

Power sockets for
camera, inner plug is
for NIR camera

Power to controller
tower

shutter

CMI | SOP003_rev1.0

Calibration

8.1

Use the silicon wafer for calibration (accepted Raman peak at 521 wavenumbers)

8.2

Choose objective to use and switch to brightfield mode (with edge filter and dichroic mirror off);
beam splitter should be in Bright Field (BF) mode (Pos 1)

8.3

Set the detector knob, at the side of binocular, to the eyepiece mode (and not the camera mode)

8.4

Set the brightness to 100% in the software (‘Illumination’). Make sure to see some intensity
changes in the video image; check it by opening and closing the aperture stop (A) at the
microscope. Typically keep this just slightly open, unless for dim samples/dic imaging.

Laser coupler

Slide rightwards(follow
arrow direction)

Options are block:

Open:

Either open , block for
633nm and 785 nm
can be chosen. All
other positions have
no filter , used for
brightfield.

Filter turret

Position 1: Brightfield
imaging

Position 2: DIC for
water dipping lens

Position 3: DIC for all
other lenses

Position 4: Raman
imaging, spectra

CMI | SOP003_rev1.0

8.5

Close the field stop and focus to bring the stage up

8.6

With the remote, select ‘Microscope Z’ control and adjust the focus (in ‘z’); when in focus
position, the image of the field stop is sharp in the video control window.

8.7

Fine tune the focus with remote observing the image of the field stop again.

8.8

Then open the field stop to observe the silicon sample.

Push/Pull rod

Fully out : light directed to

detector system

Fully in : light directed to

eyepiece camera

Eyepiece camera

Aperture stop

Field stop

Up/down: toggle
between z control, xy
stage control

X Y Stage controls

Z Stage controls

+Z : stage moves
away from objective

-Z: stage moves
towards objective

Speed control :
applies to either xy
or z. rotate white
circle anticlockwise
to reinitiate control
and increase by
rotating clockwise

Changing fibres: gently slide

the cover over the fibre and

rest on side of stand , ensuring

no kinks in fibre, unscrew the

fibre and change to the other

one. Align the raised edge on

the fibre coupling with the slot

on the fixed end then tighten

(hand tight-do not

overtighten)

Replace the black cover

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8.9

Select the correct Video Viewer (objective) in the Video Control Window and calibrate (using
‘Video Calibration’ button). The rotation should be within -1 and +1 degree. If not, rotate the
camera in the binocular and redo the calibration. Hint: center a piece of dirt or scratch in the
video viewer window and try calibration again if having trouble getting the rotation below 1.

8.10

Turn the roller (at the Raman coupler) to needed laser wavelength (with edge filter off) and
switch on the shutter of the respective laser with minimum power. Adjust the laser power until
the laser spot can be seen in the video image. Move the microscope in ‘z’ to focus the laser until
the laser spot is sharp.

8.11

Select ‘Probe position’ on the laser spot.

8.12

Make sure the correct spectrometer is connected with the camera fibre and the right laser is
selected using the ‘Configuration’ in the taskbar

50 micron fibre : 633nm use

100 micron fibre : 785nm use

It is recommended to calibrate with silicon , if switching between wavelengths, but can be

possible as a quick check just to swap in the fibre cables.

Note: Take extreme care when

handling the fibre cables as they can be damaged very easily. Ensure that the raised edge on

the fibre end lines up with slot on the connector before tightening.

8.13

Switch the coupler to laser wavelength with edge filter on.

8.14

Pull out the knob to ‘Camera mode’ (the light propagates through the detection fibre now).

8.15

Remove the beam splitter (set to either position 4) (not BF nor DIC or position 2 (extra DIC optics
filters in that position).

8.16

Start ‘Oscilloscope’, and adjust the power of the laser to get maximum intensity of the 1

order

Raman band of Silic

on at ≈520 rel.cm

-1

8.17

Adjust fine focus.

8.18

Using the X and Y fibre knob (on top of the laser coupler), get the maximum intensity of the
Raman band; then again adjust the Z focus with objective.

8.19

Redo the above steps till maximum intensity is obtained.

8.20

Record the spectrum for silicon , say 0.5 integration time , verify that the peak intensity is as
expected and in the right place ie 520 rel wavenumbers.

8.21

Close the laser shutter and stop the oscilloscope. Alignment of the microscope is now completed.

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Raman Measurements:

9.1

For

in-vitro

samples, the cells can be imaged with 633 nm laser and the nanoparticles with 785

nm laser. Saliva, to date has been recorded using 785 nm excitation.

9.2

After point scan or line scan to confirm the SERS signal from Raman reporter, an area of interest
is marked in the bright-field image.

9.3

Using ‘Sum’ filters, a spectrum region of interest can be marked; images specific to that range
will then be mapped by the WITec software. More than one range can be selected, and thus
more than one large area scan images can be constructed from a single large area scan. Eg, For
cells, vibrational bands of C-H stretching around 700 and 1000 wavenumbers can be used for
mapping.

9.4

After selecting the large area scan images with better contrast (between cells and nanoparticles),
data analysis – background correction, cosmic ray removal, basis analysis – can be performed on
large area scan data.

Configuration
display

Project window all
operations
performed during
the course of this
instance of the
software are stored
here. Rename all
files to meaningfull
names rather than
system generated
names .

Video
window
brightfield
mode

Probe position
indicator

Data processing drag
and drop operations

Indication of z
control conditions
only – doesn’t do
much

Turn on
illumination
and click auto
brightness

Hardware status window

Check
speed of
xy stage

Calibrate
video image
button

Set probe
position
button

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Troubleshooting

10.1

If you cannot see the laser spot – Check if the laser is turned on. Check if the shutter is open.

10.2

If you cannot see the white light – Check if the white light source is turned on (Illumination in
software. If it is turned on, then check if the microscope is set in Raman Mode. If it is in Raman
mode then change it to the eye-camera mode.

10.3

If you see the spectra with full of noise signal – Check for the CCD temperature. It should be
-60

C .

Shut Down Procedure

11.1

You can save the experiment parameters for your own scanning recipe by clicking “Save

Project’ in ‘File’.

11.2

Close the laser shutter, switch off the laser power supply.

11.3

Using the remote control, move the sample away from the objective.

11.4

Open the doors. Remove the sample from the stage

11.5

Discard cover slips and glass sides in the red sharps container. This includes BioHazard material.

11.6

CLEAN UP the workplace, and leave it better than you found it.

11.7

Close the software, it will take several minutes to warm up the CCD before the software

fully closes. Log-off the computer. Log out from computer, complete log book.

CMI | SOP003_rev1.0

12. APPENDIX A - CERTIFICATION: DEMONSTRATION OF SKILLS

Name:

Operation:

Date:

Tested by:

DEMONSTRATION of SKILLS

Pass Fail

Demonstrate system/ software start up and configuration

Demonstrate loading a sample on the microscope

Demonstrate finding the sample, optimizing acquisition and taking spectra

Demonstrate changing the fibre cable during the measurement session

Demonstrate finishing and shutting down system

SAFETY

Where are cover slips, glass slides discarded?

Where are biological samples discarded?

Correct use of lasers and proper handling procedures?

VALIDATION

Certification:

Pass:

Fail:

Trainee

Certified by:

Date:

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