Biological Imaging Core Facility - Centrum Nowych Technologii : Centrum Nowych Technologii

The CeNT’s Biological Imaging Core Facility is a newly established specialised laboratory dedicated to visual examination and analysis of a range of biological processes on a number of different biological systems. Currently, the lab is equipped with an upright laser scanning confocal microscope (Zeiss LSM700).

Zeiss LSM700 Confocal microscope features:

upright microscope Axio Imager Z2 mounted on antivibration table

epifluorescence imaging is provided using Metal Halide lamp source (120W) with 4 filter cubes for: DAPI, FITC/Alexa 488/Cy2/eGFP, TEXAS RED/Alexa 568/alexa 594 and Cy5

a range of lenses dedicated for brightfield and fluorescence imaging modes: 10x and 20x dry lenses, 40x and 63x oil lenses

four lasers for fluorescence excitation at 405nm, 488 nm, 555nm, 639nm

a standard detection system composed of 2 PMT detectors and a transmitted light detector allowing for simultaneous imaging up to 4 channels

spectral detection at 1nm resolution with a variable secondary dichroic (VSD) mirror which serves as a beamsplitter to direct selected wavelength band sinto separate PMT detectors

fast image acquisition up to 5 fps at 512x512 pixels

image output up to 2048x2048 pixels

dedicated Zeiss ZEN software package with a Smart Setup feature allowing for automatic microscope setup

Olympus IX73 fluorescence microscope features:

inverted microscope Olympus IX73 mounted on antivibration table

epifluorescence imaging is provided using Metal Halide lamp source (200W) with 5 filter cubes for: DAPI; FITC/Alexa Fluor 488/Fluo3/Oregon Green; Alexa Fluor 555; mCherry/Alexa Fluor 568/Alexa Fluor 594; Cy5/Alexa Fluor 647

lenses dedicated for brightfield, phase contrast and fluorescence imaging: 20x air LWD (NA 0.45) and 60x oil (NA 1.35)

in-built magnification changer allowing for additional magnification change factor of 1x, 1.6x and 2x

motorised stage with a joystick allowing for automated image acqusition and large area imaging (tile imaging and „stitching”)

high sensitivity emCCD camera (Photometrics) with a low background level suitable for live imaging

image output up to 512 x 512 pixels

dedicated Olympus cellSens Dimension software featured with multidimensional image acquisition, analysis and data processing

Nikon Eclipse fluorescence microscope features:

upright microscope Nikon Eclipse Ni-U

epifluorescence imaging is provided using Metal Halide lamp source (200W) with 4 filter cubes for: DAPI; FITC; TRITC; Cy5

a range of lenses dedicated for brightfield, phase contrast and fluorescence imaging: 4x, 10x, 20x, 40x air lenses and 40x oil immersion lens

motorised stage with a joystick allowing for precise sample navigation and large area imaging

high sensitivity digital CCD camera Retiga2000R (QImaging) with RGB colour filter allowing for up to 32bit colour digitisation

image output up to 1600 x 1200 pixels

dedicated ImagePro Plus software featured with multidimensional image acquisition, analysis and data processing

Research projects at CeNT UW realized at the Biological Imaging Core Facility:
Laboratory of Molecular Basis of Synaptic Plasticity led by Magdalena Dziembowska The aim of this project is to visualize and analyze impaired synaptic connections on hair cells in the Fmr1KO, a mouse model of the Fragile X Syndrome (FXS). The FXS syndrome is caused by a lack of expression of the fragile-X mental retardation protein (FMRP) that is involved in multiple steps of mRNA metabolism in neurons. Clinical features of FXS phenotype include intellectual disability, social communication deficit and also exhibit hypersensitivity for acoustic stimuli. The problems with acoustic information processing observed in the Fmr1KO mutant mice, as well as in the FXS patients, were thoroughly investigated in the auditory cortex in the brain. It has been hypothesized that at least part of the phenotype can be associated with the deficits of synapses located at the sensory hair cells of the organ of Corti. For confocal visualizations immunofluorescence staining with antibodies that are characteristic markers of the pre- and postsynaptic side of the ribbon synapse has been performed. The images acquired with a confocal microscope allowed for finding differences in the ribbon synapse in the Fmr1KO mice, when compared to the wild type controls.
Laboratory of Molecular and Cellular Signaling led by Paweł Niewiadomski The LSM700 confocal microscope is used for high-resolution imaging of proteins localized in primary cilia. Cilia are tiny projections on the cell surface that play the role of cellular antennae and accumulate signaling molecules. The aim of this study is to investigate how cilia are able to capture and maintain high concentrations of large proteins, such as the Gli transcription factors. The image shows the overexpressed protein Ubxn10 (green) accumulating around and inside the primary cilium (stained using anti-acetylated tubulin antibody - red). DAPI-stained nuclei are shown in blue.
Laboratory of Molecular Neurobiology led by Marta Barbara Wiśniewska While the Wnt pathway effectors Lef1, Tcf7l2 and Tcf7 are most highly expressed in the diencephalon during neurogenesis and in postmitotic cell, the role of Wnt signaling in brain development has been extensively studied mainly at earlier stages. To investigate the function of the Lef1/Tcf transcription factors in the maturation of the diencephalon, gene knockout and silencing techniques together with chemical Wnt inhibition in Danio rerio have been used. Afterwards, anatomical alterations and changes in marker gene expression in Danio rerio larvae, by double fluorescent in situ hybridization and immunochemistry have been identified.

1. What is the maximum scan penetration depth of my sample?

It very much depends on the lens used and its effective working distance (WD).
Low power dry objectives (10x or 20x) have longer working distance (5.2 mm and 0.55 mm, respectively) and thus allow for deeper penetration in a range of hundreds of microns but compromising resolution. High power objectives (40x and 63x oil immersion with WD of 0.21 mm and 0.19 mm, respectively) have much thinner scan penetration depth in a range of tens of microns but with high resolution.

2. What is the minimum/maximum thickness of my sample?

It is generally recommended to prepare thin samples (up to 100 μm) for high resolution confocal imaging. If your sample is thicker it will be still possible to scan it on the system but with more laser scattering and thus lower resolution.

3. Is your system suitable for live imaging?

Unfortunately, our confocal system is not equipped with a dedicated environmental chamber which limits the possibility of live imaging of biological specimens.

4. What laser lines are available for fluorescence excitation?

The system comes with 4 diode laser lines: 405nm (5mW), 488nm (10mW), 555nm (10mW), 639nm (5mW)

5. What are the possible experimental applications of your system?

Our system allows for a number of different applications including 3D visualisations and reconstructions, time lapse experiments combined with photoactivation/photobleaching e.g. FRAP or FRET, channel unmixing for clear spearation of overlapping peaks, co-localisation analyses, spectral imaging (lambda scanning) etc. You can find some examples of recent applications under the „Research” tab.

6. What is the maximum resolution you can achieve with your system?

The maximum theoretical spatial resolution in laser scanning confocal microscopy is diffraction-limited according to the following equation:

Resolution (r) = 0.61λ/NA, where λ – imaging wavelength, NA – numerical aperture of the objective

In practical terms, a resolution limit of ~200-300nm in xy and ~700-800nm in z can be achieved using a short laser wavelength of 405nm. This can be further affected by other factors such as sample thickness, sample density, sensitivity to photobleaching etc.

7. What are the microscope scanning modes?

The microscope works in two basic modes – epifluorescence and reflection.
In epifluorescent mode, the laser excites fluorescence within the sample – this is either natural fluorescence (autofluorescence) or a fluorescent dye that has been attached to a specific site on the sample using an antibody label.

In reflection mode the laser light is simply bounced off the surface of the specimen allowing for additional information from specimens that reflect light or have significant fluctuations of refractive index at certain boundaries e.g. to study various cell-matrix interactions.

8. What is the maximum size of a sample?

As long as the sample fits on a single slide it can be imaged even on a macro scale by automatic tiling of individual frames. The stage of our system accommodates up to 10 individual microscopic slides which can be all loaded at the same time.

9. What is the minimum step size of your stage?

Our stage is fully motorised with a travel range in XY of 225 x 85 mm and a minimum step size in Z of 10nm.

10. How do I need to prepare my samples prior to my confocal session?

Your sample preparation protocol is very much dependent on the sample type. It is recommended to mount it on a standard microscopic slide (76x26mm) with a coverslip on top. The samples can be mounted in a solution buffer or other media e.g. glycerol or glycerine and ideally should be immobilised to avoid unwanted movements during acquisition. For more tips and tricks please fill the form in the „Client Zone” section.

11. What is the average time for generating results for commercial samples?

The time depends on the number of samples and experiment type. Typically, a high resolution Z stack acquisition of a 50um thick sample takes up to 1 hour including microscope setup. A half-day confocal session is enough to scan up to 5 samples with high resolution.

12. Can we set a non-disclosure agreement for my commercial research?

Yes, that is possible.

13. How do I get access to my data after finishing my session?

Your data are saved as raw .czi files and will be backed up on the CeNT’s server after each session. They can be then downloaded offline to your memory drive from dedicated CeNT’s workstations.

14. What is the average throughput time needed to process a batch of samples per week?

Depending on the experiment type, we can image and process approximately 10-20 samples per week but this is all arranged on an individual basis once we know more details of the research needs.

15. Is it possible to use your system for a collaborative project?

Absolutely. We are an open access facility and welcome any potential collaborators to conduct their experiments at CeNT UW. Such visitors (if external to UW) will be charged a preferential academic rate compared to fully commercial users. For a full price list please refer to the „Pricelist” tab.

16. What is the average waiting time to analyse my samples?

The microscope is available to all interested users and as such can be quite busy from time to time. However, the average time to book a session should be less than 2 weeks. You can check the current reservation status in the „Client Zone” tab.

17. Is it possible to discuss my research needs or sample preparation protocol before booking an instrument time?

Certainly yes. It is our priority to understand your needs or assist you in a sample preparation step prior to actual microscopy time. We allow our users to fully describe their requirements by filling in an online form in the „Client Zone” tab. This can serve as a good starting point for some face-to face discussions before deciding on the experimental time and post-processing data analysis.

Internal users (unassisted use)	32 PLN/h	8 €/h	10 $/h
External academic users (assisted use)*	150 PLN/h	40 €/h	45 $/h
External non-academic users (assisted use)*	225 PLN/h	55 €/h	60 $/h

Prices include tax.
* For Zeiss LSM 700 Confocal microscope only

A formal acceptation of the rules and regulations is required prior to granting access to core facilities equipment and staff consultations. All information about them you can find in the form below:Ładuję…

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Zeiss LSM 700

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Olympus IX73

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Nikon Eclipse fluorescence microscope

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Internal User Order Form to be completed and signed by internal CeNT/UW users prior to making reservation assignments.

Formularz zamówienia wewnętrznego użytkownika

External User Order Form to be completed and signed by external academic or external non-academic users prior to making reservation assignments.

Formularz zamówienia zewnętrznego użytkownika

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