Dear all,
Two postdoctoral positions are currently available in the structural
biology laboratory of Dr. Zhiyi Wei (http://bio.sustc.edu.cn/en/?p=189) at
Department of Biology, Southern University of Science and Technology
(SUSTech, Shenzhen, China). Our research interests is to uncover
to continue refinement?
> Eleanor
> On 30 Jul 2012, at 09:27, Zhiyi Wei wrote:
>
>> Dear all,
>>
>> I have a refine structure with 8 ncs copies and several hundreds of
>> water molecules (which was put in one chain). Now I try to separate
>> these molecules by
Dear all,
I have a refine structure with 8 ncs copies and several hundreds of
water molecules (which was put in one chain). Now I try to separate
these molecules by renaming to the chain id of each adjacent protein
molecule. I know RCSB can do this during deposition process. Do anyone
know a progr
Hi Leonid,
Thank you for your valuable suggestion. It is exactly the case. When I
tried P21, it works well. The solution is now very clear.
Best,
Zhiyi
On 3/31/12, Leonid Sazanov wrote:
> Hi, we had the same case in apparent C2221, with many similarly shifted
> Phaser solutions with high scores
Dear all,
I got a weird solution from Phaser. The background is that, space
group C2221, resolution ~4A, in complex with a peptide, and having a
apo form structure as the search model. Phaser gave two rotation
function peaks with Z > 7. But when searching translation function
peaks, Phaser gave ma
Hi Yuan,
Bad geometry is a general issue for most low resolution structure
refinement. There are quite a lot papers discussing it. I think you
can try to set a reference structure or set high restrain in
refinement, which should be easily achieved in Phenix. How did you
know the B-factors are too
ons where
> multiple "single crystal domains" are collected. The same applies if you
> apply translations at the crystal (to collect data from fresh crystal
> regions to decrease the radiation damage effect).
>
> Hope it helps, cheers,
>
> Carlos
>
>
> Zhiyi W
TH
>
> Jens
>
>
> On Wed, 2012-01-04 at 21:42 +0800, Zhiyi Wei wrote:
>> Dear all,
>>
>> I recently collected a dataset (~2000 frames) from a single crystal.
>> If merge first 600 frames (sca1) or last 600 frames (sca2), Rmerge
>> values from scalepack
Dear all,
I recently collected a dataset (~2000 frames) from a single crystal.
If merge first 600 frames (sca1) or last 600 frames (sca2), Rmerge
values from scalepack seem to be ok (~10%) though rejection ratios are
high (~5%). But if I merge all frames together, Rmerge value goes up
to ~20% and
Dear all,
I am trying to refine a structure with two domains. The electron
density of one domain is reasonable, but that of the other domain is
poor. So, I am wondering whether the refinement by Phenix or Refmac
can be done locally with two parts, the first domain is refined with
normal restrains,
!
Zhiyi
On Wed, Jun 8, 2011 at 11:20 AM, Clemens Vonrhein
wrote:
> Hi,
>
> try
>
> reindex hklin in.mtz hklout out.mtz < REIN HKL -h,-k,l
> END
> e
>
> Cheers
>
> Clemens
>
> On Wed, Jun 08, 2011 at 11:14:03AM -0400, Zhiyi Wei wrote:
>> Dear all
Dear all,
I have a P2 derivative dataset with beta=89.6. I try to change the
beta to 90.4 to be consistent with the native dataset. Should I do sth
with the HKL, like applying a matrix? Thanks a million!
Best,
Zhiyi
Dear all,
Our group plan to buy a X-ray diffraction system. We found Bruker
provide a new X-ray generator called Microstar, which they claim is
better than traditional rotating anode tube. Because we did not use
Microstar before, we do not know whether this new generator is indeed
good choice in r
Depending where you are - they might have the equipment to do
>>
>> a wet mount - without freezing. Yes the crystal will not last - but
>> then you know if the problem is in the
>> crystal. If it is - you need better crystals. If it is the cryo - you
>> need to wor
diffraction pattern is
similar.
On Tue, Jan 26, 2010 at 10:42 AM, Zhiyi Wei wrote:
> Dear all,
>
> I got a problem with my crystals. I have two total different proteins
> that both can be crystallized in the condition with PEG3350 and Tacsimate
> (although the concentrations are different)
Hi everyone,
I want to know which ATP analogues are suitable and popular for
co-crystallization
with enzyme.
Thank you in advance.
Best,
Zhiyi
--
Zhiyi Wei
-
Institute of Biophysics, Chinese Academy of Sciences
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