Zeiss Axio-Observer spinning-disk microscope

J-A Bombardier Building, Room 3223-1 Advanced Microscope Tier 2 usage price
Instrument awarded to Dr. Daniel Zenklusen by the Canadian Foundation for Innovation (CFI)

Applications
- Transmitted light
- Fluorescence
- Live-cell imaging
- Incubator (Temperature & CO₂)

·         Light sources
o    LED for transmitted light
o    Lumencor SOLA for visible fluorescence
Lumencor SOLA complete specifications

Emission peak (nm)	Power (mW)
334	5
365	20
405	19
436	22
546	21
579	18

o 4 lasers 405, 488 561 638
Laser complete specifications

Laser line (nm)	Nominal Power (mW)
405	50
488	100
561	50
639	50

·         Objectives
1.      100x/1.46 Oil WD 0.11
2.      TIRF Divergence adjusting aid

TIRF Angle adjusting aid

4.      63x/1.46 Oil WD 0.1
5.      10x/0.3 Air WD 5.2
6.      Empty
Full lens specifications

Position

Nom

Marque

Nom complet

Identifiant

Grossissement

Ouverture numérique

Immersion

Type

Distance de travail (mm)

Transmittance
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Technique

Épaisseur du couvre-objet (mm)

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1

100x/1.46 Oil

Zeiss

100x/1.46 DIC I
Alpha Plan-ApoChromat
M27

420792-9800

100x

1.46

Oil

Plan Apochromat

0.11

>70% [410-800]

BF, DIC, Fluo

0.17

2

TIRF Divergence adjusting aid

Zeiss

423682-8801-000

3

TIRF Angle adjusting aid

Zeiss

423682-8802-000

4

63x/1.46 Oil

Zeiss

63x/1.46 DIC III
Alpha Plan-Apochromat Korr TIRF
M27

420780-9970-000

63x

1.46

Huile

Plan Apochromat

0.10

>80% [500-800]

BF, DIC, Fluo

0.15-0.19

5

10x/0.3 Air

Zeiss

10x/0.3 EC Plan-NeoFluar

420340-9901

10x

0.3

Air

Plan-NeoFluar

5.2

>90% [450-750]

BF, DIC, Fluo

0.17

6

Empty

BF: Bright-field DIC: Interference contrast

· Filter cubes

Empty
BS_455
LSM TFT80/20 1447-381
BF RL TIRF Calibration 424928
Set 76 C/G/Dr
Set 77 G/R/A6

7. Complete filter specifications

Position	Nom	Marque	Identifiant	Filtre d'excitation	Miroir dichroïque	Filtre d'émission	Commentaire
1	Empty
2	BS_455	Zeiss			455LP		To be used with FRAP 405
3	LSM Duo T20/R80 UV	Zeiss
4	Brightfield Ref Light	Zeiss
5	Set 76 CFP GFP DsRed	Zeiss	489076-0000-000	390-422 484-501 549-573	427 503 578	448-472 512-538 585-631
6	Set 77 GFP/RFP/Alexa633	Zeiss	489077-0000-000	469-497 552-577 629-650	506 582 659	510-542 587-614 665-711

Detector
- 2 EMCCD camera Photometrics Evolve 512 x 512 pixels, 16-bit, 33 f/s at full resolution, sensor size 8.192 mm x 8.192mm, pixel size 16um x 16um Evolve512-Datasheet.pdf Evolve512_Manual.pdf

Startup

Turn on the computer (#1)
If required, turn on the incubation power bar

3.      Turn on the camera and laser power bar on the left of the microscope (#2)
4.      Turn on the microscope power bar on the right of the microscope (#3)
5.      Use your UdeM credentials to log in to Windows
When using for the first time, it is necessary to import the microscope-specific parameters BEFORE starting the software. See the First Use section below.
6.      Start the Zen Blue software
First Use
When using for the first time, it is necessary to import the microscope-specific parameters into the software. This procedure is usually carried out during the training session. However, it is also possible to use it to reset the software if it is not displayed correctly, for example.
Please note, this procedure will delete all your experiment protocols and restore the software to its original settings.

If open, close the Zen Blue software and wait for it to close completely (up to 30 seconds)
On the Desktop open the Documentation folder
Double-click Settings for Axio-Observer Z1
A script will run and a black window will appear briefly
You can then reopen the Zen Blue software

Loading samples
This procedure puts the microscope in a safe configuration and performs a focus calibration. At the end of this procedure the microscope will be ready for acquisition.
Focus Calibration Z
On the microscope touch screen:

Press Home>Load Position to lower the stage to its lowest position
Press Set Work Position to store this position
If necessary, move the focus slightly up to remove the "Lower Z limit reached" message displayed on the touchscreen
Press Home>Microscope>Turret>Objectives>10x to select the 10x objective
If asked, tap Done to remove the oil lens cleaning warning
Press Home>Microscope>XYZ>Position>Z-Position>Set zero>Auto to perform focus calibration
Press OK to start the focus calibration procedure
Wait a few seconds for the calibration to be completed

Once calibrated, the focus can be found at Z = 5 mm). The Z value can be found on the microscope touch screen Home>Z-Position
First focus
Make sure to calibrate the focus before performing the first focus.
On the microscope touch screen:

Press Home>Microscope>Turret>Objectives
Press 10x to select the 10x lens

The 10x objective is the safest because it has the longest working distance (5.3 mm). The sample will appear perfectly sharp long before the lens approaches it. It is recommended to always first focus with the safest lens. The objectives are para-focal, focusing with the safest objective will then allow you to easily find your sample with another objective.

Press Home>Load Position to lower the stage to its lowest position
Press Set Work Position to store this position
If necessary, move the focus slightly up to remove the "Lower Z limit reached" message displayed on the touchscreen
Place the test slide on the microscope stage with the coverslip toward the objective

Always use the test slide to perform the first focus.

If necessary, move the stage so that the sample is centered on the objective

On the computer:

Open the Zen Blue software
In the Locate tab, select BF or the desired fluorescence ((CFP/GFP/DsRed ou GFP/RFP/Cy5, etc…) to activate the configuration
Adjust the focus with the main dial while looking through the eyepieces until the image is perfectly sharp

Once calibrated, the focus can be found at Z = 5 mm). The Z value can be found on the microscope touch screen Home>Z-Position

In the Locate tab, select Off to turn off the illumination

Seconday focus
Important
First focus with the safest lens before selecting another lens and continuing with secondary focus.
Focusing with air objectives
This microscope does not have additional air objectives. However, if there were, the procedure would be as follows:
After performing the first focus, on the microscope touch screen:

Press Home>Microscope>Turret>Objectives
Press on the desired lens

In Zen Blue software:

In the Locate tab, select BF or the desired fluorescence (CFP/GFP/DsRed ou GFP/RFP/Cy5, etc…) to activate the configuration
Adjust the focus with the precision dial while looking through the eyepieces until the image is perfectly sharp
In the Locate tab, select Off to turn the illumination off
Your sample is ready for acquisition!

Focusing with oil lenses
After performing the first focus, on the microscope touch screen:

Press Home>Microscope>Turret>Objectives

2. Press 63x Oil (1.4) or 100x Oil (1.4) to select the desired lens. The microscope will automatically lower the stage so that the sample is accessible.
The 63x objective is the best oil objective because it has the most optical corrections (Plan Apochromat) and the largest numerical aperture (1.4). It offers a lateral resolution of 240nm at a wavelength of 550nm.

Remove your sample from the microscope
Place a drop of oil on the objective
Replace your sample from the microscope
Press Done. The microscope will automatically return the sample to its original position

In Zen Blue software:

In the Locate tab, select BF or the desired fluorescence (CFP/GFP/DsRed ou GFP/RFP/Cy5, etc…) to activate the configuration
Adjust the focus with the precision dial while looking through the eyepieces until the image is perfectly sharp
In the Locate tab, select Off to turn the illumination off
Your sample is ready for acquisition!

Storage management

Files can be saved temporarily (during acquisition) on the local C: drive (desktop)
At the end of each session, copy your data to your external drive and delete it from the local C: drive
You can store your files on the D: drive (Data Storage). If you do, please create a folder per laboratory using the principal investigator last name. Within, create one folder per user (Firstname_Lastname).

In any case, your files should be removed from the C: drive.
Shutdown

Save your data
Close the software Zen Blue
Transfer your data to the D: drive (Data Storage) or to your external drive and delete it from the local C: drive
If used, turn of the incubation power bar
If used, clean oil lenses with lens cleaner and paper

6. Turn off the microscope power bar on the right of the microscope (#3)

Turn off the camera and laser power bar on the left of the microscope (#2)
Turn off the computer

Important Reminders

Take back your samples including ones in the microscope
Leave the microscope and the working area clean

The following diagrams allow you to follow the light path in transmitted light (bright field, DIC) and in reflected light (fluorescence).

Zen quick start guide.pdf

To do
Check Loss of 488nm laser power
2024-04-26
(FIXED) Problem with the FRAP module:
At first could not modulate the laser intensity (yet could not find the spot on the field), rebooted and then the FRAP fiber does not carry any light (even 488)
==> Laser manipulation module was too far in x and y (noticeable as a tilt and a gap between both parts of the module).
2024-03-04
Corrected Trigger Module configuration for the BackCam

reassigned each camera with its own trigger module in MTB config

2024-02-29

DualCam calibration parameters set, using beads
Realigned Lasers:
- Laser output measured in spinning disk mode at the sample with 10x objective, 1x Extended tubelens, 100% laser power and ALL lasers ON:
  - 405nm: 0.70 mW before => 0.66 mW after
    - with laser 488 OFF: 0.81 mW before => 0.83 mW after
  - 488nm: 3.75 mW before => 4.17 mW after
    - with laser 405 OFF: 3.95 mW before => 4.33 mW after
  - 561nm: 2.1 mW before => 2.37 mW after
  - 639nm: 0.9 mW before => 1.1 mW after
NOTE: AOTF2 for FRAP

AOTF2 calibration
For FRAP, the illumination is strongest with the AOTF2 at 60% and not 100%
· Error message when switching between FRAP & SD illumination
AOTF2 Error message
FRAP/SD illumination switching triggers an error message " 'MTBAOTF2LaserLine6' is not supported by the current hardware"
2021-11-20

Zen 2.6 updated hotfix 12
Microsoft Windows update
Laser output measured in spinning disk mode at the sample with 10x objective, 1x Extended tubelens, 100% laser power and ALL lasers ON:
- 405nm: 1.08 mW StdDev 0.01mW

o 488nm: 3.3 mW StdDev <0.01mW (3.7 mW if laser 405 is OFF)
405nm and 488nm Interactions
When both 405nm and 488nm laser are ON simultaneously, the output power is decreased by 11%.

- 561nm: 2.6 mW StdDev <0.01mW
- 639nm: 1.37 mW StDev 0.02 mW

· Control for vibrations during construction work on the 4th floor
2021-11-03

Error when the definite focus is used (unexpected error the definite focus did not respond)
To solve it:
- Turn off the Zen Software
- Turn off the microscope power bar (#3)
- Turn off the definite focus by pressing and holding the definite focus button
- Turn on the definite focus by pressing once the definite focus button
- Wait until the definite focus display shows "Detecting stand"
- Turn on the microscope power bar (#3)
Confirm that the definite focus is showing in the microscope tactile display
Open Zen software and run an experiment using the definite focus to confirm it is fully functional

2021-09-27

Added to wiki

2020-07-07

AOTF1 changed

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