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Apotome Guide

1) The ApoTome uses a moving grid and software to generate images that exclude out-of-focus light, allowing finer structures to be seen more clearly compared to standard fluorescent images. 2) Calibration must be done for each objective and filter set using a calibration slide, and involves focusing the grid lines and optimizing the image. 3) Additional calibration is needed for each fluorescent marker, using the sample slide, to configure the ApoTome settings for that marker.

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Putut D. Utomo
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150 views

Apotome Guide

1) The ApoTome uses a moving grid and software to generate images that exclude out-of-focus light, allowing finer structures to be seen more clearly compared to standard fluorescent images. 2) Calibration must be done for each objective and filter set using a calibration slide, and involves focusing the grid lines and optimizing the image. 3) Additional calibration is needed for each fluorescent marker, using the sample slide, to configure the ApoTome settings for that marker.

Uploaded by

Putut D. Utomo
Copyright
© © All Rights Reserved
We take content rights seriously. If you suspect this is your content, claim it here.
Available Formats
Download as PDF, TXT or read online on Scribd
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QueenslandBrainIns#tuteMicroscopy

ApoTome:UsersGuide
Op#calSec#oningwithApoTome
ApoTomeusesamovinggridtochangehowtheslideisilluminated.Bytakingseveralimages,withthegridin
dierentposi#ons,theApoTomeso?wareisabletogenerateasingleimagewhichexcludesalargeamountofthe
outoffocuslighttypicallypresentinuorescentimages.
Theresul#ngimageslookcrisperthanthesmootherstandarduorescentimage,whichallowsnerstructuresand
detailstobeseenclearlybuttheyarealsodimmer(asthereislesslightreachingthecamera).

GFP

GFPwithApoTome

Calibra#ngApoTome

Calibra#onmustbecarriedseparatelyforeachobjec#veandlterset.
1.InsertthecorrectgridintotheApoTomeslider
AxioImager:
5x,10x,and20xobjec#ve=Lgrid
40x,63xand100x=Hgrid
AxioObserver:
5xand10x=Lgrid
40x=Dgrid
20xand63x=Hgrid
1. UnlockandremovetheApoTomesliderfromthesideofthemicroscope.
2. Usethetweezerstogentlyremoveandinserttheappropriategrid.
Wheninser#ng,matchupthewhitedotonthegridwiththeoneontheslider.
Thegridisheldinmagne#callysoifitsnotsiXnglevelmoveitaroundslightlywiththetweezers
un#litclicksintoplace.
Onceinplacecheckitissecurebyli?ingthesliderandgentlytappingitoverthepalmofyour
hand.
3. ReturntheApoTomesliderbackintothemicroscope
Therearetwostopposi#ons.Allthewayin/1stclick(forusingApoTome/grid)ortheclick
before2ndclick(fornormalimaging/iris).
WhenyounishusingApoTomeremembertopullthesliderbackouttothe2ndclick/iris
posi<on.
QueenslandBrainIns#tuteMicroscopy

Calibra#ngApoTome
2.PhaseCalibraAon
Thiscalibra#onrequiresthemirroredcalibraAonslide.
1. Focusonthecrosshairatthecentreofthesilversquareonmirroredcalibra#onslide.
EnsureyouareusingtheBFRL(brighEieldreectedlight)ltersetandtheHXPlamp.
Thelightshiningontheslideshouldappearyellowgreenanddowntheeyepiecesthecrosshair
shouldappearblack.
2. Onceyouhavefoundthecrosshairswitchtocameramodeandensurethecrosshairisfocusedasbest
youcan.
IfthecrosshairisoutoffocusyouwillnotcalibrateApoTomecorrectly.

OutofFocus

CorrectlyFocused

3. InthetopmenugotoAcquisiAon>ApoTome>PhaseCalibraAon
4. Inthewindowthatappearsmakesureyouhavetherightobjec#veselected,thecorrectgridsizeselected
andthatyouareusingtheBFRLlter.
5. ClickNext.
6. Nowadjusttheexposureofthecameraforimagingthecrosshair.Itshouldadjustautoma#callyby
clickingmeasure.Ifnot,bringtheexposureofthecameratoapointwherethereismaximumbrightness
butnooverexposure.
7. ClickNext.
8. PushtheApoTomesliderallthewayintothemicroscope.Youshouldbe
abletoseegridlinesacrosstheliveimage.
9. Leavetheexposureasitisandposi#onthegreenrectangleoveranarea
containingroughly10gridlines.Thisistheareaaxiovisionwilllookatto
automa#callyfocusonthegridlines.
Makesuretherectangleisnotoverthecrosshair.
10. ClickFullScan.

11. TheGridwillmovethroughaseriesofposi#ons,un#litndsaposi#on
wherethegridlinesareinfocus.Thegraphshowingtheposi#onsshould
haveadenedpeakatthebestloca#on.
IfthereisnodenedpeakApoTomeisnotcalibraAngcorrectly.

QueenslandBrainIns#tuteMicroscopy

Calibra#ngApoTome
12. ClickLocalScantoensureaxiovisionhasfoundthebestgridposi#on.OncethisiscompleteclickNext.
13. Thissteprequiresyoutostraightenthecamera.Movethestageslightlysothatthecrosshaircannotbe
seenthengentlytwistthecameraun#lyoutheanglereads0.0(orascloseaspossible).

14. ClickNext.
15. YouwillnowneedtodoanotherFullScan.IfApoTomeisworkingcorrectlythegraphwilllooksimilarto
below.OncecompleteclickLocalScan,thenclickNext.

16. Thephasecalibra#onisnownished.Ifyouchangeobjec#vesyouwillneedtocalibrateforthenew
objec#ve.
3.GridFocusCalibraAon
Thiscalibra#onstepistocongureApoTomeforeachuorescentmarkeryouareusing.
1. RemovethemirroredcalibraAonslideandfocusonyoursampleslide.
2. UnderthedropdownmenugotoAcquisiAon>ApoTome>GridFocusCalibraAon.
3. Therstwindowthatappearsallowsyoutochoosewhichltersetyouwishtocalibratefor(e.g.FITCor
DsRed).YoudonotneedtochangeanyoftheotherseXngshere.Selecttheappropriatelterandclick
Next.
4. AdjusttheexposurebyclickingMeasure,thenclickNext
5. PushtheApoTomesliderintoplacethegridshouldbefaintlyvisibleovertheuorescenceofyour
sample.

QueenslandBrainIns#tuteMicroscopy

Calibra#ngApoTome

6. Drawthegreenselec#onrectangleoverabrightregionoftheimage(thiswillhelpaxiovisionfocusthe
grid).OnceyouhaveselectedabrightareaclickFullScan.
Ifyoucantseethegridlinesduringthefullscan,eitherthesampleistoodimforApoTome,or
ApoTomeisnotcalibraAngcorrectly.
Ifithascalibratedyouwillseeadenedpeakandthegridlineswillbevisibleontheimage.

7. OnceyouhavecompletedtheLocalScanclickNext.
8. ApoTomeisnowcalibratedforthismarker.Youwillneedtorunthiscalibra#onagainforeachuorescent
markeryouareusing.
Itisnecessarytocreateanewcalibra#onforeachmarkerbutalsoforeachlightsource(i.e.
separatecalibra#onswillberequiredtoexciteGFPwiththecolibriLEDsandtheexternalHXP
lamp).

ImportantSeXngsforApoTome
ClickonApoTomeintheworkareatothele?.UndertheseYngstabselect:
1. Thecorrectgridfortheobjec#vebeingused.
2. TheGridVisibleop#onunderLiveModethiswillensurethefastest
refreshrateforlivemode
3. TheOpAcalSecAoningop#onunderAcquisi#onModeifnotchecked
op#calsec#oningwillnotoccur
4. AweakApoTomelterisrecommendedifgridlinesares#llvisibleinthenal
imaged.Thislterisusedtoremoveanybandsle?bythegridsbutagood
calibra#onshouldavoidthis.
5. 2xAveraging(noisereduc#on)isrecommendedasanini#alseXng.Youmay
notneedthisifyoursampleisbright,likewisemayneedtoincreasethiswith
par#cularlydimsamples.
UndertheextrastabensurethedisplaynormalizaAonboxis#cked.
ApoTomeimagesareverydimasmostofthelightisbeingremoved
DisplayNormalisa#onrescaleshowtheimagesaredisplayedsoyoucan
seethemproperly.
IfyouareusingApoTomebutyourimagesappearcompletelyblackthis
op#onismostlikelydisabled.

OnceApoTomehasbeencalibratedyoucanimageasnormal(e.g.usingLive/Snapor
MulAdimensionalAcquisiAonexperiments).ApoTomeopAcalsecAoningwilloccurwheneverthe
ApoTomesliderispushedallthewayintothemicroscope.
QueenslandBrainIns#tuteMicroscopy

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