LISTSERV - CONFOCALMICROSCOPY Archives

CONFOCALMICROSCOPY Archives

January 2011

CONFOCALMICROSCOPY@LISTS.UMN.EDU

	LISTSERV Archives
	CONFOCALMICROSCOPY Home
	CONFOCALMICROSCOPY January 2011

	Log In
	Register

	Subscribe or Unsubscribe

	Search Archives

Options:	Use Monospaced Font Show Text Part by Default Show All Mail Headers
Message:	[<< First] [< Prev] [Next >] [Last >>]
Topic:	[<< First] [< Prev] [Next >] [Last >>]
Author:	[<< First] [< Prev] [Next >] [Last >>]

Subject:	Re: Indo with multiphoton question
From:	"José A. Feijó" <[log in to unmask]>
Reply To:	[log in to unmask]
Date:	Thu, 13 Jan 2011 00:02:50 +0000
Content-Type:	text/plain
Parts/Attachments:	text/plain (113 lines)

*****
To join, leave or search the confocal microscopy listserv, go to:
http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
*****

we did it for proof of principle, fig. 28 in
Feijó & Moreno, 2004, Imaging plant cells by two-photon 
excitation,Protoplasma, 223:1-32

(also attached)

basically Paul is on spot (as usual)

Em 07-01-2011 20:17, Paul Herzmark escreveu:
> *****
> To join, leave or search the confocal microscopy listserv, go to:
> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
> *****
>
> Hi Michael,
>
> We do it here with the laser tuned to 720. We separate the two Indo peaks
> into two different PMTs by using a 440 dichroic. The emission light going to
> the short wave PMT also goes through a 400/45 bandpass filter. The light to
> the long wave PMT goes through a 480/50 bandpass filter.
>
> Hope that helps!
>
> Paul
>
>
> Paul Herzmark
> Specialist
> [log in to unmask]
>
> Department of Molecular and Cell Biology
> 479 Life Science Addition
> University of California, Berkeley
> Berkeley, CA  94720-3200
> (510) 643-9603
> (510) 643-9500 fax
>
>
> On Fri, Jan 7, 2011 at 9:12 AM, Cammer, Michael
> <[log in to unmask]>wrote:
>
>> *****
>> To join, leave or search the confocal microscopy listserv, go to:
>> http://lists.umn.edu/cgi-bin/wa?A0=confocalmicroscopy
>> *****
>>
>> Dear multiphotoners,
>>
>> I'm planning to try using Indo on the multiphoton microscope next week and
>> was wondering whether anybody has tips on best wavelengths to use for
>> excitation (e.g. 720 or 920 nm?) or anything else of potential use.
>>
>> Thank you!
>>
>> Sincerely,
>>
>> Michael
>>
>> ________________________________________________________
>> Michael Cammer, Assistant Research Scientist
>> Skirball Institute of Biomolecular Medicine
>> Lab: (212) 263-3208  Cell: (914) 309-3270
>>
>> </PRE>
>> <html>
>> <body>
>> ------------------------------------------------------------<br />
>> This email message, including any attachments, is for the sole use of the
>> intended recipient(s) and may contain information that is proprietary,
>> confidential, and exempt from disclosure under applicable law. Any
>> unauthorized review, use, disclosure, or distribution is prohibited. If you
>> have received this email in error please notify the sender by return email
>> and delete the original message. Please note, the recipient should check
>> this email and any attachments for the presence of viruses. The organization
>> accepts no liability for any damage caused by any virus transmitted by this
>> email.<br />
>> =================================
>> </body>
>> </html>
>> <PRE>
>>
> .
>

-- 


**********************************************************
Jose' A. Feijo', Prof.
----------------------------------------------------------
Dep. Biologia Vegetal, Fac.Ciencias, Universidade Lisboa
PT-1749-016 Lisboa, PORTUGAL

tel. +351.21.750.00.47/00/24, fax  +351.21.750.00.48

and/ e

Inst.Gulbenkian Ciencia, PT-2780-156 Oeiras, PORTUGAL

tel. +351.21.440.79.41/00/19, fax +351.21.440.79.70
__________________________________________________________
e.mail: [log in to unmask]  or  [log in to unmask]

URL: http://www.igc.gulbenkian.pt/research/unit/38
or   http://dbv.fc.ul.pt/users/jafeijo

**********************************************************

ATOM RSS1 RSS2

LISTS.UMN.EDU