Zeiss AxioImager.Z2 Fluorescence Protocol

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Zeiss AxioImager.Z2 Fluorescence Protocol 1) System Startup Please note put sign-up policy. You must inform the facility at least 24 hours beforehand if you can t come; otherwise, you will receive a charge for unused time. The facility will allow for extenuating circumstances (cells dying, sick day, etc.) if you inform us in a timely fashion. Follow each step of the startup poster and wait for the microscope software to fully load. 2) Lens Cleaning Please clean all of the lenses (used and unused) before and after your session. Refer to the lens cleaning poster if you need any help recalling the rules and steps. 3) Microscope Control Take note of the microscope light path: A. Light source B. Direction through microscope C. Filter G D. Lens E. Slide a. Since we are measuring reflected light, you will C B A not use the optics below the stage F. Lens G. Camera/ Eyepiece F D a. Note the locking positions of the sliders and remember to be delicate! The slider pulls E glass. Touch pad control Within the Home menu, select Microscope and then Turret (Stay within this window for the entire session and ignore other tabs) Objective Menu: always begin focusing using the 10x lens. Page 1 of 9

(a) Take care to properly set your focal position with the lower power lens before going to a higher power lens. Proper focusing from low power to high power will help prevent the microscope from breaking your slide. Reflector Menu: select your first filter channel To open the shutter, turn the RL illumination on the far right of the screen On (a) Remember to close the shutter as often as you open it to prevent rapid bleaching of your sample. (b) Note: The active option is always white. Always begin imaging with the 10x objective and take care for the following issues: Select and inspect each slide If it is dirty, gently clean with a Kim Wipes and/or cotton swab. You should do this with all your slides before you come. Load the slide securely into the stage clip. Focusing will become difficult when the slide is uneven. Joystick Control Use the joystick to find your region of interest Use the F1 button in the upper right to toggle between course and fine x and y control Page 2 of 9

Focus Control Course and fine focus control are located on both sides of the microscope. If you are focusing on the right side of the microscope, the fine focus is located INSIDE the coarse focus. You can adjust by using the finger positions within the coarse. FINE Focus your sample and check all the channels before imaging. 4) Software Control Open the Zen Software Select the Zen Pro imaging option Click Skip calibration Upon Zen s completed startup, please note the 3 divisions of the interface: Left: control panel Middle: Top: image preview and acquired image Page 3 of 9

Bottom: display options Right: image gallery Preview Window Control Panel Image Gallery Display Window 5) Your first image Gently push both sliders all the way in to send the light to the eyepiece. Use the touchpad to: Select the 10x lens in the objective menu Select your first filter channel and open the shutter in the reflector menu Use the stage movement wand and focus knob to focus and center your specimen on a region of interest. Be sure to check all fluorophores in your specimen. You need to have an idea of what to expect before imaging with the camera. Use the touchpad RL illumination option to close the shutter. Pull the TOP camera/eyepiece slider out to send light to the camera. Page 4 of 9

1 2 6 3 Active focus control 5 4 Within the Zen software: Setup your experiment in the Control Panel: AVOID THE LOCATE TAB! Click the Acquisition tab Select the Channels window. Choose the wavelengths by checking channel names. (Channels are listed by descending wavelengths.) Make your most important channel your focus reference by clicking on the channel until it turns gray, and select Focus Ref. In the Live mode, focus on the reference channel. Focus using the computer keyboard Page 5 of 9

Put your cursor over the image and hit Ctrl on the keyboard; use the mouse roller to fine tune the focus (to signify focus activation, a dialog box will appear). Focus using the microscope fine focus Click Range Indicator at the bottom of the screen. Click Set Exposure within the channels window. Click Stop (the same icon as Live ) Click the remaining channels and set exposure times. When all exposure times are set, Click Snap to acquire the image. Image Saving Options: Click the Save As button to save the image in your directory within the specified User Data folder. Note: All data is stored in the D: drive under the User Data folder. Be sure to save to the User Data folder and NOT the Users folder. Optional: Auto-save function Note: There is also an auto save function that must be enabled AND disabled before and after your session. You CANNOT export overlay images using this tool. Save raw.czi file Save tiff files Use the same parameters from the batch protocol to export your single channel images. Page 6 of 9

6) Higher magnification and switching slides If you switch to the higher magnification oil immersion lenses from a dry immersion lens, go back to the microscope and enter the objective menu on the touchpad. Press the high power lens you want to use. The lens will then move to the correct objective and the stage will drop. The touchpad will prompt you to put immersion on the specimen. At this point, apply one drop of oil and click Done to raise the stage back up. If you switch from an oil lenses to a dry lens, after the touchpad prompts you to remove the immersion, take the slide out, wipe off the oil with a cotton swab. Replace the slide into the stage clip and click Done to raise the stage back up. When you need to switch slides, Go back to the 10x and refocus the new sample If you are imaging a similar sample using the same objective lens, click the Load Position button located in the upper right hand corner of the touchpad. This will allow you to lower the stage, replace your slide with a new one, and restore the same focal plane. Page 7 of 9

7) Data Export Go to the Processing tab (located to the right of the Acquisition tab) Click Batch Under Batch Method select Image Export In the middle of the screen under Batch Processing, click Add and then select all the images you want to export. Highlight one image Under parameters, make the following selections File type: Tagged Image File (.tiff) Compression: None Unclick convert to 8 bit Check Use Full Set of Dimensions Unclick Create project folder unless you would like all images in separate folders Exporting options: also within the parameters tab, you can choose the display of your images Select Orignal Data to export the raw data in gray Select Individual Channel Images to export the individual channels with pseudocolor Select Merge Channels Images to export the overlay (a) Note: All image display types CAN be exported at the same time. (b) Note: You can batch several groups of images differently and run them simultaneously. 1 2 3 Underneath Batch Processing, Click Copy Parameters Select all images. (Ctrl +Shift A) Click Paste Parameters Click Run Selected Page 8 of 9

8) System Shutdown Back up all your data. Clean all the lenses. Check the microscope calendar to see when the next user has an appointment If the user comes within 2 hours, log off your account Otherwise, follow shutdown poster steps. Page 9 of 9