rking in a cold room to harvest your crystals will help reduce the
evaporation rate.
Good luck!
Best,Anna
On Tue, Jul 10, 2012 at 9:28 AM, m zhang wrote:
regaentDear All,
I am sure this question was discussed before. But I am wondering if anyone got
the same experience as I do. I got a
You could also try high salt solutions with similar technique.
Good luck!
Jim
From: CCP4 bulletin board [CCP4BB@JISCMAIL.AC.UK] on behalf of m zhang
[mzhang...@hotmail.com]
Sent: Tuesday, July 10, 2012 11:28 AM
To: CCP4BB@JISCMAIL.AC.UK
Subject: [ccp4bb] cryo for high salt
regaentDear All,
I am sure this question was discussed before. But I am wondering if anyone got
the same experience as I do. I got a crystal out of condition with 1M KCl, 1.4M
Ammonium sulfate at pH7. I tried to use glycerol, ethylene glycol, 25% sucrose,
paraton-N oil, or ammonium sulfate itse
e e-mail and do not disclose its contents to
any person. Any unauthorized review, use, disclosure, copying or distribution
is strictly prohibited.Von: CCP4 bulletin board [mailto:CCP4BB@JISCMAIL.AC.UK]
Im Auftrag von m zhang
Gesendet: Freitag, 16. September 2011 04:20
An: CCP4BB@JISCMAIL.AC.UK
Dear all,
I have two questions:
First, I was trying to crystallize a complex of two proteins. Both proteins has
been crystallized before. The two proteins bind to each other based on Biacore
study, but they didn't form a single peak on gel filtration. When I mixed them
at 1:1 ratio, the cry
this helps.
Regards,
Krishna
Krishna Chinthalapudi
Graduate Student
Hannover Medical School
Germany
On Thu, Aug 4, 2011 at 4:32 AM, m zhang wrote:
Dear all,
I have two unrelated questions. Any suggestion on any of them will be greatly
appreciated.
First, we have two proteins
Dear all,
I have two unrelated questions. Any suggestion on any of them will be greatly
appreciated.
First, we have two proteins that bind each other without a doubt. But since we
have very limited amount of proteins and it takes a long time to reproduce
them, we are very hesitating to try
Dear all,
I am trying to optimize my crystal with additives. Since the yield of my
protein purification is very limited, I am wondering what is the most efficient
way to set up drops with additive to save my protein and not wasting additives?
I am setting up 1 to 1 drops with 0.2 ul additiv
example,
temperature, cuture, etc.
Best,
Lin
On Fri, Jan 21, 2011 at 8:12 PM, m zhang wrote:
Dear All,
Recently I am trying to express a glycoprotein in Drosophila S2 cells. However,
the expression yield is every low and most of the protein expressed aggregate.
I was suggested making new
Dear All,
Recently I am trying to express a glycoprotein in Drosophila S2 cells. However,
the expression yield is every low and most of the protein expressed aggregate.
I was suggested making new constructs. But I am wondering if anyone here can
give me some suggestions to improve it beyond tha
Hi All,
I was trying to make a model-mask file for ncs-averaging in DM. I noticed
that in CNS, the mask file has to be O-compressed. Does that mean if I read in
O the mask file and write it out, the output file is already in O-compressed
format?
Related to the first question, the second on
Hi everyone,
I have some basic questions about CNS. First, I am wondering if there is
anywhere I can set my initial B-factor during my early refinement. When I
generate my initial model in generate.inp, I can set the B-factore. However,
after I did the rigid.inp and anneal.inp, the B-factor just
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