BasicsCoursePhDprog-PeterEvennetOct2011-observed timing and needed materials
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* First day Handout for students | * First day Handout for students | ||
* Light torches | * Light torches | ||
− | + | * cameras and monitors | |
+ | * Cleaning stations for each table | ||
+ | * condenser screwdrivers for each microsocpe | ||
+ | * oil/DIC objectives for each microscope (next to stand) | ||
+ | * 2 polarization filters for each microscope | ||
=== DAY ONE (24th Oct)=== | === DAY ONE (24th Oct)=== | ||
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− | |style="background:LemonChiffon;"|15: | + | |style="background:LemonChiffon;"|15:50 |
− | |style="background:LemonChiffon;"| | + | |style="background:LemonChiffon;"|17:05 || align="center" style="background:LemonChiffon;"|SESSION 2<br>Practice<br> (30min Rotation)|| align="center" style="background:LemonChiffon;"|conjugate planes on Peters microscope <br> conjugate planes on optical bench||align="center" style="background:LemonChiffon;"|PETER EVENNETT<br>JAN ||align="center" style="background:LemonChiffon;"| *Peters microscope setup <br> *optical bench demonstrating a transmitted light microscope, incl. light source |
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− | | | + | |17:05||17:25||align="center"|SESSION 3<br>Theory||align="center" |Koehler Illumination <br> (Microscope alignment)||align="center" |PETER EVENNETT || |
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|} | |} | ||
− | === DAY TWO ( | + | === DAY TWO (25th Oct)=== |
{| border="4" cellpadding="2" cellspacing="8" {| {{table}} | {| border="4" cellpadding="2" cellspacing="8" {| {{table}} | ||
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| align="center" style="background:#f0f0f0;"|'''Materials needed''' | | align="center" style="background:#f0f0f0;"|'''Materials needed''' | ||
|- | |- | ||
− | | 9:00||10:00||align="center"|Recap ||align="center" | day 1 ||align="center" |LMF TEAM | + | | 9:00||10:00||align="center"|Recap ||align="center" | day 1 ||align="center" |LMF TEAM || align="center" | Questions |
|- | |- | ||
|- | |- | ||
− | + | | 10:00||10:45||align="center"|SESSION 1<br>Theory||align="center" | Epi-Illumination <br> Lens aberrations and corrections ||align="center" |PETER EVENNETT || | |
− | | | + | |
− | | | + | |
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|-- | |-- | ||
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− | | style="background:mediumseagreen;"|''' | + | | style="background:mediumseagreen;"|'''10:45''' |
− | | style="background:mediumseagreen;"|'''11: | + | | style="background:mediumseagreen;"|'''11:00''' |
|align="center" style="background:mediumseagreen;"|'''BREAK''' | |align="center" style="background:mediumseagreen;"|'''BREAK''' | ||
− | |align="center" style="background:mediumseagreen;"|'''COFFEE BREAK'''|| align="center" style="background:mediumseagreen;"|''Note: have break earlier next time, right after diffraction-string-show <br> (should be shortly before 11am)<br>then do all the explanation of Abbe's Diffraction Exp after break'' | + | |align="center" style="background:mediumseagreen;"|'''COFFEE BREAK'''|| align="center" style="background:mediumseagreen;"|''Note: have break earlier next time, right after diffraction-string-show <br> (should be shortly before 11am)<br>then do all the explanation of Abbe's Diffraction Exp after break'' ||align="center" style="background:mediumseagreen;" | |
|- | |- | ||
− | | 11: | + | | 11:00||12:45||align="center"|Session 2 <br> Theory & DEMONSTRATION || align="center"|Diffraction and Diffraction slide fun <br> Diffraction string show <br> ABBE'S DIFFRACTION EXPERIMENT<br>Peter's Video (50min) ||align="center"|PETER EVENNETT || align="center" | Diffraction slides, torch, "dashed" string |
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− | | style="background:mediumseagreen;"|'''12: | + | | style="background:mediumseagreen;"|'''12:45''' |
− | | style="background:mediumseagreen;"|'''13: | + | | style="background:mediumseagreen;"|'''13:45''' |
|align="center" style="background:mediumseagreen;"|'''BREAK''' | |align="center" style="background:mediumseagreen;"|'''BREAK''' | ||
− | |align="center" style="background:mediumseagreen;"|'''LUNCH'''|| style="background:mediumseagreen;"|''' ''' | + | |align="center" style="background:mediumseagreen;"|'''LUNCH'''|| style="background:mediumseagreen;"|''' ''' ||align="center" style="background:mediumseagreen;" | |
|- | |- | ||
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− | | 13: | + | | 13:45||14:35||align="center"| SESSION 3<br>Demo and Theory || align="center"| Dan's setup demonstration ||align="center" |DAN ||align="center" |Dan's ABBE Diffraction demo setup |
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− | | 14: | + | |style="background:LemonChiffon;"| 14:35 |
+ | |style="background:LemonChiffon;"|15:00||align="center" style="background:LemonChiffon;"|SESSION 1 <br>Theory & Practice||align="center" style="background:LemonChiffon;"| Depth of Field<br>Depth of Focus ||align="center" style="background:LemonChiffon;"|PETER EVENNETT <br>LMF TEAM || align="center" style="background:LemonChiffon;"| students microscopes with 10x/0.25 and 40x/0.65 objectives <br> Stereoscope with a "sample" | ||
|- | |- | ||
|- | |- | ||
− | | style="background:mediumseagreen;"|''' | + | | style="background:mediumseagreen;"|'''15:00''' |
− | | style="background:mediumseagreen;"|'''15: | + | | style="background:mediumseagreen;"|'''15:20''' |
|align="center" style="background:mediumseagreen;"|'''BREAK''' | |align="center" style="background:mediumseagreen;"|'''BREAK''' | ||
− | |align="center" style="background:mediumseagreen;"|'''COFFEE BREAK'''|| style="background:mediumseagreen;"|''' ''' | + | |align="center" style="background:mediumseagreen;"|'''COFFEE BREAK'''|| style="background:mediumseagreen;"|''' ''' ||align="center" style="background:mediumseagreen;" | |
|- | |- | ||
|- | |- | ||
− | | 15: | + | | 15:20 || 15:55 ||align="center"|SESSION 4<br>Theory|| align="center"| Dark Field microscopy||align="center" |PETER EVENNETT || |
|- | |- | ||
|- | |- | ||
|style="background:LemonChiffon;"| 15:55 | |style="background:LemonChiffon;"| 15:55 | ||
− | |style="background:LemonChiffon;"| 16:30 ||align="center" style="background:LemonChiffon;"|SESSION 4<br>Practice|| align="center" style="background:LemonChiffon;"|Dark Field microscopy||align="center" style="background:LemonChiffon;"|LMF TEAM | + | |style="background:LemonChiffon;"| 16:30 ||align="center" style="background:LemonChiffon;"|SESSION 4<br>Practice|| align="center" style="background:LemonChiffon;"|Dark Field microscopy||align="center" style="background:LemonChiffon;"|LMF TEAM || align="center" style="background:LemonChiffon;"| diatome slides |
|- | |- | ||
|- | |- | ||
− | | 16:30||16:50||align="center"|SESSION 5<br>Theory|| align="center"|Basics of Phase Contrast microscopy ||align="center" |PETER EVENNETT | + | | 16:30||16:50||align="center"|SESSION 5<br>Theory|| align="center"|Basics of Phase Contrast microscopy ||align="center" |PETER EVENNETT || |
|- | |- | ||
|- | |- | ||
|style="background:LemonChiffon;"| 16:50 | |style="background:LemonChiffon;"| 16:50 | ||
− | |style="background:LemonChiffon;"|17:30||align="center" style="background:LemonChiffon;"|SESSION 5<br>Practice|| align="center" style="background:LemonChiffon;"|Phase Contrast microscopy ||align="center" style="background:LemonChiffon;"|LMF TEAM | + | |style="background:LemonChiffon;"|17:30||align="center" style="background:LemonChiffon;"|SESSION 5<br>Practice|| align="center" style="background:LemonChiffon;"|Phase Contrast microscopy ||align="center" style="background:LemonChiffon;"|LMF TEAM || align="center" style="background:LemonChiffon;"| cheek cell samples |
|- | |- | ||
|- | |- | ||
− | | 17:30|| : ||align="center"|SESSION 5<br>Theory|| align="center"|Details of Phase Contrast microscopy ||align="center" |PETER EVENNETT | + | | 17:30|| : ||align="center"|SESSION 5<br>Theory|| align="center"|Details of Phase Contrast microscopy ||align="center" |PETER EVENNETT || |
|} | |} | ||
− | + | === DAY THREE (26th Oct)=== | |
− | === DAY THREE ( | + | |
{| border="4" cellpadding="2" cellspacing="8" {| {{table}} | {| border="4" cellpadding="2" cellspacing="8" {| {{table}} | ||
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| align="center" style="background:#f0f0f0;"|'''Materials needed''' | | align="center" style="background:#f0f0f0;"|'''Materials needed''' | ||
|- | |- | ||
− | | 9:00||10:00||align="center"|Recap ||align="center" | day 2 ||align="center" |LMF TEAM | + | | 9:00||10:00||align="center"|Recap ||align="center" | day 2 ||align="center" |LMF TEAM || align="center" |Questions |
|- | |- | ||
− | | 10:00||10: | + | | 10:00||10:45||align="center"|SESSION 1<br>Theory||align="center" | Objective reading<br>eye pieces||align="center" |PETER EVENNETT <br>LMF TEAM || align="center" |objectives, eyepieces, polylux |
|- | |- | ||
|- | |- | ||
− | | style="background:mediumseagreen;"|'''10: | + | | style="background:mediumseagreen;"|'''10:45''' |
− | | style="background:mediumseagreen;"|''' | + | | style="background:mediumseagreen;"|'''11:00''' |
|align="center" style="background:mediumseagreen;"|'''BREAK''' | |align="center" style="background:mediumseagreen;"|'''BREAK''' | ||
− | |align="center" style="background:mediumseagreen;"|'''BREAK'''|| align="center" style="background:mediumseagreen;"|'''BREAK''' | + | |align="center" style="background:mediumseagreen;"|'''BREAK'''|| align="center" style="background:mediumseagreen;"|'''BREAK''' || align="center" style="background:mediumseagreen;" | |
|- | |- | ||
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− | |style="background:LemonChiffon;"| | + | |style="background:LemonChiffon;"| 11:00 |
− | |style="background:LemonChiffon;"|12: | + | |style="background:LemonChiffon;"|12:30||align="center" style="background:LemonChiffon;"|SESSION 1<br>Practice<br>Group rotation (30min. each!)||align="center" style="background:LemonChiffon;"| Cover glasses and sample mounting<br>Objective reading<br> Objective cleaning||align="center" style="background:LemonChiffon;"|Dan<br>Britta, Silke<br>Jan ||align="center" style="background:LemonChiffon;"| Coverglasses (High preciscion), different oils <br> 8-10 different, "interesting" objectives (for a group of 4-5) <br> slides, oils, different cleaning reagents |
|- | |- | ||
|- | |- | ||
− | | 12: | + | | style="background:mediumseagreen;"|'''12:30''' |
+ | | style="background:mediumseagreen;"|'''13:30''' | ||
+ | |align="center" style="background:mediumseagreen;"|'''BREAK''' | ||
+ | |align="center" style="background:mediumseagreen;"|'''LUNCH'''|| style="background:mediumseagreen;"|''' ''' || style="background:mediumseagreen;"|''' ''' | ||
|- | |- | ||
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− | | | + | | 13:30||14:00||align="center"|SESSION 2<br>Theory||align="center" | Polarized light microscopy||align="center" |PETER EVENNETT || |
− | | | + | |
− | |align="center | + | |
− | |align="center | + | |
|- | |- | ||
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|style="background:LemonChiffon;"| 14:00 | |style="background:LemonChiffon;"| 14:00 | ||
− | |style="background:LemonChiffon;"|14:40||align="center" style="background:LemonChiffon;"|SESSION 2<br>Practice||align="center" style="background:LemonChiffon;"| Polarized light microscopy||align="center" style="background:LemonChiffon;"|LMF TEAM | + | |style="background:LemonChiffon;"|14:40||align="center" style="background:LemonChiffon;"|SESSION 2<br>Practice||align="center" style="background:LemonChiffon;"| Polarized light microscopy||align="center" style="background:LemonChiffon;"|LMF TEAM|| align="center" style="background:LemonChiffon;"| Hair, stone samples, benzocain cristals, rulers, gummi bears, plastic dishes, ... |
|- | |- | ||
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− | | 14:40||15:05||align="center"|SESSION 3<br>Theory|| align="center"|Differential Interference Contrast (DIC)||align="center" |PETER EVENNETT | + | | 14:40||15:05||align="center"|SESSION 3<br>Theory|| align="center"|Differential Interference Contrast (DIC)||align="center" |PETER EVENNETT || |
|- | |- | ||
|- | |- | ||
|style="background:LemonChiffon;"| 15:05 | |style="background:LemonChiffon;"| 15:05 | ||
− | |style="background:LemonChiffon;"|15:40||align="center" style="background:LemonChiffon;"|SESSION 3<br>Practice|| align="center" style="background:LemonChiffon;"|Differential Interference Contrast (DIC)||align="center" style="background:LemonChiffon;"|LMF TEAM | + | |style="background:LemonChiffon;"|15:40||align="center" style="background:LemonChiffon;"|SESSION 3<br>Practice|| align="center" style="background:LemonChiffon;"|Differential Interference Contrast (DIC)||align="center" style="background:LemonChiffon;"|LMF TEAM|| align="center" style="background:LemonChiffon;"| cheek cell samples |
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| style="background:mediumseagreen;"|'''16:00''' | | style="background:mediumseagreen;"|'''16:00''' | ||
|align="center" style="background:mediumseagreen;"|'''BREAK''' | |align="center" style="background:mediumseagreen;"|'''BREAK''' | ||
− | |align="center" style="background:mediumseagreen;"|'''BREAK'''|| align="center" style="background:mediumseagreen;"|'''BREAK''' | + | |align="center" style="background:mediumseagreen;"|'''BREAK'''|| align="center" style="background:mediumseagreen;"|'''BREAK'''|| align="center" style="background:mediumseagreen;"| |
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− | |||
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− | | 16: | + | | 16:00||17:10||align="center"|SESSION 4a<br>Theory & Demo|| align="center"|What is a pixel<br>Analog to Digital conversion<br>Nuyquist-Shannon||align="center" |Dan || |
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− | |style="background:LemonChiffon;"| 17: | + | |style="background:LemonChiffon;"| 17:10 |
− | |style="background:LemonChiffon;"| | + | |style="background:LemonChiffon;"|17:30||align="center" style="background:LemonChiffon;"|SESSION 3<br>Practice|| align="center" style="background:LemonChiffon;"|PIXELS||align="center" style="background:LemonChiffon;"|LMF TEAM ||align="center" style="background:LemonChiffon;"| Sesame seeds, sunflower seeds, nudels, gumibears and a checker board |
+ | |- | ||
+ | |- | ||
+ | | 17:30||18:00||align="center"|SESSION 4b<br>Theory & Demo|| align="center"|Spatial Calibration and more||align="center" |Dan || | ||
+ | |- | ||
+ | |- | ||
+ | | 18:00|| ||align="center"|Question round|| align="center"|Questions to Peter Evennett||align="center" |PETER EVENNETT <br>LMF TEAM || | ||
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|} | |} | ||
− | === DAY FOUR ( | + | === DAY FOUR (27th Oct)=== |
{| border="4" cellpadding="2" cellspacing="8" {| {{table}} | {| border="4" cellpadding="2" cellspacing="8" {| {{table}} | ||
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− | | 14:00||15:45||align="center"|SESSION 3<br>Theory & Practice|| align="center"|Imaging with CCD and Quantitative Imaging ||align="center" |LMF TEAM<br> Britta/Dan||align="center" | • CCD<br> • Cameras || align="center" |• CCD chip <br> • RGB Slider Spot Camera setup | + | | 14:00||15:45||align="center"|SESSION 3<br>Theory & Practice|| align="center"|Imaging with CCD and Quantitative Imaging ||align="center" |LMF TEAM<br> Britta/Dan||align="center" | • CCD<br> • Cameras || align="center" |• CCD chip <br> *example cameras showing different chip sizes <br> • RGB Slider Spot Camera setup |
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| style="background:mediumseagreen;"|'''15:45''' | | style="background:mediumseagreen;"|'''15:45''' | ||
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|align="center" style="background:mediumseagreen;"|'''BREAK'''|| style="background:mediumseagreen;"|''' '''|| style="background:mediumseagreen;"|''' '''|| style="background:mediumseagreen;"|''' ''' | |align="center" style="background:mediumseagreen;"|'''BREAK'''|| style="background:mediumseagreen;"|''' '''|| style="background:mediumseagreen;"|''' '''|| style="background:mediumseagreen;"|''' ''' | ||
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− | | 16:00||18:00||align="center"|SESSION 4<br>Practice|| align="center"|Imaging with CCD cameras using LMF systems ||align="center" |LMF TEAM ||align="center"|• Displaying <br>• Pixel size<br>• Look up table<br>• Binning<br>• Exposure time<br>• Saturation<br>• Signal to noise <br>• ROI<br>• Bit depth<br>• Auto map<br>• Auto contrast || align="center"|• Microscopes: <br> DVcore(Dan, 3 students)<br> | + | | 16:00||18:00||align="center"|SESSION 4<br>Practice|| align="center"|Imaging with CCD cameras using LMF systems ||align="center" |LMF TEAM ||align="center"|• Displaying <br>• Pixel size<br>• Look up table<br>• Binning<br>• Exposure time<br>• Saturation<br>• Signal to noise <br>• ROI<br>• Bit depth<br>• Auto map<br>• Auto contrast || align="center"|• Microscopes: <br> DVcore(Dan, 3 students)<br> N-Storm (Britta, 3 students)<br> Inverted CCD (Pete, 2 students)<br> self-built-syst (Jan, 3 students)) <br>• Fluorescence Sample slides (Kidney / Cells) |
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'' | '' | ||
− | === DAY FIVE ( | + | === DAY FIVE (28th Oct)=== |
{| border="4" cellpadding="2" cellspacing="8" {| {{table}} | {| border="4" cellpadding="2" cellspacing="8" {| {{table}} | ||
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| align="center" style="background:#f0f0f0;"|'''Materials needed''' | | align="center" style="background:#f0f0f0;"|'''Materials needed''' | ||
|- | |- | ||
− | | 9:00||10: | + | | 9:00||10:30||align="center"|Recap ||align="center" | day 4 ||align="center" |LMF TEAM||align="center"|Question sheets (!) |
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− | |||
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− | + | | style="background:mediumseagreen;"|'''10:30''' | |
− | | style="background:mediumseagreen;"|''' | + | | style="background:mediumseagreen;"|'''10:45''' |
− | | style="background:mediumseagreen;"|''' | + | |
|align="center" style="background:mediumseagreen;"|'''BREAK''' | |align="center" style="background:mediumseagreen;"|'''BREAK''' | ||
− | |align="center" style="background:mediumseagreen;"|'''BREAK'''||align="center" style="background:mediumseagreen;"|'''BREAK''' | + | |align="center" style="background:mediumseagreen;"|'''BREAK'''||align="center" style="background:mediumseagreen;"|'''BREAK'''||align="center" style="background:mediumseagreen;"| ''note: break might have been too early? (usually in between the Optical sectioning talk)'' |
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− | | | + | |10:45||13:00||align="center"|SESSION 1<br>Theory & Demo||align="center" | Optical sectioning methods<br>Pros&Cons ||align="center" |LMF TEAM <br> Dan / Jan ||align="center" |"confocal equipment": <br> laser pointer, mirror, broken scanning mirror <br> dual laser pointer (green and red) to demonstrate penetration of diff. wavelength |
− | + | ||
|- | |- | ||
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| style="background:mediumseagreen;"|'''13:00''' | | style="background:mediumseagreen;"|'''13:00''' | ||
| style="background:mediumseagreen;"|'''14:00''' | | style="background:mediumseagreen;"|'''14:00''' | ||
− | |align="center" style="background:mediumseagreen;"|''' | + | |align="center" style="background:mediumseagreen;"|'''LUNCH''' |
− | |align="center" style="background:mediumseagreen;"|'''LUNCH'''|| style="background:mediumseagreen;"|''' | + | |align="center" style="background:mediumseagreen;"|'''LUNCH'''|| align="center" style="background:mediumseagreen;"|'''LUNCH'''|| style="background:mediumseagreen;"| |
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− | | 14:00||15:00||align="center"|SESSION 2<br>Small Groups Discussion|| align="center"|What techniques might be good for me<br> (Own Projects) ||align="center" |LMF TEAM<br>Dan/Jan/Silke/Britta/Pete? | + | | 14:00||15:00||align="center"|SESSION 2<br>Small Groups Discussion|| align="center"|What techniques might be good for me<br> (Own Projects) ||align="center" |LMF TEAM<br>Dan/Jan/Silke/Britta/Pete?||align="center" | |
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| style="background:mediumseagreen;"|'''15:15''' | | style="background:mediumseagreen;"|'''15:15''' | ||
|align="center" style="background:mediumseagreen;"|'''BREAK''' | |align="center" style="background:mediumseagreen;"|'''BREAK''' | ||
− | |align="center" style="background:mediumseagreen;"|'''BREAK'''|| align="center" style="background:mediumseagreen;"|'''BREAK''' | + | |align="center" style="background:mediumseagreen;"|'''BREAK'''|| align="center" style="background:mediumseagreen;"|'''BREAK'''|| align="center" style="background:mediumseagreen;"| |
|- | |- | ||
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− | | 15:15||16:00||align="center"|SESSION 3|| align="center"|Course evaluation ||align="center" |LMF TEAM | + | | 15:15||16:00||align="center"|SESSION 3|| align="center"|Course evaluation ||align="center" |LMF TEAM||align="center" | |
|} | |} |
Latest revision as of 11:46, 28 October 2011
Contents |
[edit] PhD Program: Basics of Light Microscopy - Peter Evennett / LMF - Course May 2011
[edit] Setup -Fri 21 Oct
Setup - all lmf staff move stuff to galleria Equipment needed
- Microscopes
- Optical bench
- Spinning disk gadget
- Polarazing sheets
- Diffraction Grids
- Fluorescent samples
- Fluorescent Beads (Prepare slides)
- First day Handout for students
- Light torches
- cameras and monitors
- Cleaning stations for each table
- condenser screwdrivers for each microsocpe
- oil/DIC objectives for each microscope (next to stand)
- 2 polarization filters for each microscope
[edit] DAY ONE (24th Oct)
FROM | TO | ACTIVITY | TOPICS | Responsible person(s) | Materials needed |
9:00 | 09:30 | FINAL PREP | Test everything works | LMF | |
9:40 | 10:25 | INTRODUCTION | COURSE INTRO WHO is WHO? Round table |
LMF TEAM | White board and pen |
10:25 | 10:55 | Session 1 Theory |
PRINCIPLES OF LIGHT MICROSCOPY Historical aspects Very basic components and principles ( incl. Refraction-basics) |
PETER EVENNETT | |
10:55 | 11:10 | BREAK | BREAK | ||
11:15 | 11:30 | SESSION 1 Practice SHORT (5min !!!) Rotation |
capillary in oil demo Coin-in-cup demo red and green laser through milky water with black background |
DAN PETER PETE & JAN |
*capillaries, oil * coin-in-cup, water *laser pointer, glass with "milky" water and black background |
11:30 | 12:45 | SESSION 1 Theory |
Introduction to lenses (Lens demo fun) Lens aberrations (see colour fringes of lighting image with simple lens) Resolution, Numerical aperture Magnification |
PETER EVENNETT | little lenses |
12:45 | 13:45 | LUNCH | LUNCH | ||
13:45 | 14:45 | SESSION 1 Practice 15min (!!!) Rotation |
Milky Glass Block demo Show and discuss microscope parts (upright and inverted) NA measurements |
DAN JAN & BRITTA SILKE |
*milky glass block, teaching microscope, coloured filters for microscope, iris objective *slides with arrows, simple upright and inverted microscope *horizontal protractor on stand, objective holder, 2 air objective with different (!) NAs (and maybe an iris objective), calculator, pencils, rubber |
14:45 | 15:30 | SESSION 2 Theory |
Microscope illumination Conjugate planes |
PETER EVENNETT | |
15:30 | 15:45 | BREAK | BREAK | ||
15:50 | 17:05 | SESSION 2 Practice (30min Rotation) |
conjugate planes on Peters microscope conjugate planes on optical bench |
PETER EVENNETT JAN |
*Peters microscope setup *optical bench demonstrating a transmitted light microscope, incl. light source |
17:05 | 17:25 | SESSION 3 Theory |
Koehler Illumination (Microscope alignment) |
PETER EVENNETT | |
17:15 | 18:30 | SESSION 3 Practice |
Koehler illumination (Microscope alignment) |
LMF TEAM | students manual microscopes, screwdrivers, nice brightfield sample |
[edit] DAY TWO (25th Oct)
FROM | TO | ACTIVITY | TOPICS | Responsible person(s) | Materials needed |
9:00 | 10:00 | Recap | day 1 | LMF TEAM | Questions |
10:00 | 10:45 | SESSION 1 Theory |
Epi-Illumination Lens aberrations and corrections |
PETER EVENNETT | |
10:45 | 11:00 | BREAK | COFFEE BREAK | Note: have break earlier next time, right after diffraction-string-show (should be shortly before 11am) then do all the explanation of Abbe's Diffraction Exp after break |
|
11:00 | 12:45 | Session 2 Theory & DEMONSTRATION |
Diffraction and Diffraction slide fun Diffraction string show ABBE'S DIFFRACTION EXPERIMENT Peter's Video (50min) |
PETER EVENNETT | Diffraction slides, torch, "dashed" string |
12:45 | 13:45 | BREAK | LUNCH | ||
13:45 | 14:35 | SESSION 3 Demo and Theory |
Dan's setup demonstration | DAN | Dan's ABBE Diffraction demo setup |
14:35 | 15:00 | SESSION 1 Theory & Practice |
Depth of Field Depth of Focus |
PETER EVENNETT LMF TEAM |
students microscopes with 10x/0.25 and 40x/0.65 objectives Stereoscope with a "sample" |
15:00 | 15:20 | BREAK | COFFEE BREAK | ||
15:20 | 15:55 | SESSION 4 Theory |
Dark Field microscopy | PETER EVENNETT | |
15:55 | 16:30 | SESSION 4 Practice |
Dark Field microscopy | LMF TEAM | diatome slides |
16:30 | 16:50 | SESSION 5 Theory |
Basics of Phase Contrast microscopy | PETER EVENNETT | |
16:50 | 17:30 | SESSION 5 Practice |
Phase Contrast microscopy | LMF TEAM | cheek cell samples |
17:30 | : | SESSION 5 Theory |
Details of Phase Contrast microscopy | PETER EVENNETT |
[edit] DAY THREE (26th Oct)
FROM | TO | ACTIVITY | TOPICS | Responsible person(s) | Materials needed |
9:00 | 10:00 | Recap | day 2 | LMF TEAM | Questions |
10:00 | 10:45 | SESSION 1 Theory |
Objective reading eye pieces |
PETER EVENNETT LMF TEAM |
objectives, eyepieces, polylux |
10:45 | 11:00 | BREAK | BREAK | BREAK | |
11:00 | 12:30 | SESSION 1 Practice Group rotation (30min. each!) |
Cover glasses and sample mounting Objective reading Objective cleaning |
Dan Britta, Silke Jan |
Coverglasses (High preciscion), different oils 8-10 different, "interesting" objectives (for a group of 4-5) slides, oils, different cleaning reagents |
12:30 | 13:30 | BREAK | LUNCH | ||
13:30 | 14:00 | SESSION 2 Theory |
Polarized light microscopy | PETER EVENNETT | |
14:00 | 14:40 | SESSION 2 Practice |
Polarized light microscopy | LMF TEAM | Hair, stone samples, benzocain cristals, rulers, gummi bears, plastic dishes, ... |
14:40 | 15:05 | SESSION 3 Theory |
Differential Interference Contrast (DIC) | PETER EVENNETT | |
15:05 | 15:40 | SESSION 3 Practice |
Differential Interference Contrast (DIC) | LMF TEAM | cheek cell samples |
15:40 | 16:00 | BREAK | BREAK | BREAK | |
16:00 | 17:10 | SESSION 4a Theory & Demo |
What is a pixel Analog to Digital conversion Nuyquist-Shannon |
Dan | |
17:10 | 17:30 | SESSION 3 Practice |
PIXELS | LMF TEAM | Sesame seeds, sunflower seeds, nudels, gumibears and a checker board |
17:30 | 18:00 | SESSION 4b Theory & Demo |
Spatial Calibration and more | Dan | |
18:00 | Question round | Questions to Peter Evennett | PETER EVENNETT LMF TEAM |
[edit] DAY FOUR (27th Oct)
FROM | TO | ACTIVITY | TOPICS | Responsible person(s) | DEMO Activities | Materials needed |
9:00 | 10:00 | Recap | day 3 | LMF TEAM | ||
10:00 | 10:45 | SESSION 1 Theory |
Fundamental concepts of fluorescence | DAN | - | - |
10:45 | 11:00 | BREAK | BREAK | BREAK | BREAK | BREAK |
11:00 | 12:15 | SESSION 2 Theory & Practice |
Fluorescence Microscopy | SILKE LMFTEAM |
• Light sources • Lamp houses • Spectra • Filters • Filter cubes • Filter spectral charts of each microscope (laminated) |
• Spare lamp houses • Lamps • Ocean optics equipment • Four (4) different Filter-sets (cubes), with the appropriate descriptions • diagramms for drawing filter/fluorophore spectra |
12:15 | 13:00 | SESSION 2 Practice |
Fluorescence imaging at microscopes | LMF TEAM | - | • Fluorescent labeled samples |
13:00 | 14:00 | BREAK | LUNCH | LUNCH | LUNCH | LUNCH |
14:00 | 15:45 | SESSION 3 Theory & Practice |
Imaging with CCD and Quantitative Imaging | LMF TEAM Britta/Dan |
• CCD • Cameras |
• CCD chip *example cameras showing different chip sizes • RGB Slider Spot Camera setup |
15:45 | 16:00 | BREAK | BREAK | |||
16:00 | 18:00 | SESSION 4 Practice |
Imaging with CCD cameras using LMF systems | LMF TEAM | • Displaying • Pixel size • Look up table • Binning • Exposure time • Saturation • Signal to noise • ROI • Bit depth • Auto map • Auto contrast |
• Microscopes: DVcore(Dan, 3 students) N-Storm (Britta, 3 students) Inverted CCD (Pete, 2 students) self-built-syst (Jan, 3 students)) • Fluorescence Sample slides (Kidney / Cells) |
19:00 | open end | Dinner | with Peter | LMF TEAM |
[edit] DAY FIVE (28th Oct)
FROM | TO | ACTIVITY | TOPICS | Responsible person(s) | Materials needed |
9:00 | 10:30 | Recap | day 4 | LMF TEAM | Question sheets (!) |
10:30 | 10:45 | BREAK | BREAK | BREAK | note: break might have been too early? (usually in between the Optical sectioning talk) |
10:45 | 13:00 | SESSION 1 Theory & Demo |
Optical sectioning methods Pros&Cons |
LMF TEAM Dan / Jan |
"confocal equipment": laser pointer, mirror, broken scanning mirror dual laser pointer (green and red) to demonstrate penetration of diff. wavelength |
13:00 | 14:00 | LUNCH | LUNCH | LUNCH | |
14:00 | 15:00 | SESSION 2 Small Groups Discussion |
What techniques might be good for me (Own Projects) |
LMF TEAM Dan/Jan/Silke/Britta/Pete? |
|
15:00 | 15:15 | BREAK | BREAK | BREAK | |
15:15 | 16:00 | SESSION 3 | Course evaluation | LMF TEAM |