Re: [AMBER] AMBER Digest, Vol 1932, Issue 1

From: Elvis Martis <elvis.martis.bcp.edu.in> Date: Tue, 6 Jun 2017 09:43:21 +0000

--
*Regards*
Garima Singh
AcSIR-PhD Fellow
Biotechnology Division
C/o Dr. Ashok Sharma (Chief Scientist and Head Biotechnology Division)
Central Institute Of Medicinal And Aromatic Plant
CSIR-CIMAP
Lucknow
garimabioinfo.gmail.com
*INDIA* Please don't print this e-mail unless you really need to. Be Green !
On Tue, May 23, 2017 at 12:47 PM, Garima Singh <garimabioinfo.gmail.com>
wrote:
>  Dear Martis ,
>              As per your previous mail, we have tried that sample script
> to run Amber, but this time error message was "command mpirun not found".
>            The modified script was
>
>
> #! /bin/csh
> #PBS -l walltime=10:00:00
> #PBS -N my_job
> #PBS -q workq
> #PBS -l select=1:ncpus=16:mpiprocs=16
> #PBS -l place=scatter:excl
> #PBS -V
>
> # Go to the directory from which you submitted the job
> cd $PBS_O_WORKDIR
>
> source /home/ashoks/amber14/amber14/amber.csh
>
> mpirun -np 16 sander.MPI -O -i Prod.in -o Prod.out -p cd_cdat7.prmtop -c
> Heat.rst -r prod.rst -x prod.mdcrd -inf prod.info &
>
> and our working directory was :  /home/ashoks/5_garima/at550l/
>
> Please do the needful.
>
>
>
>
>
>
>
>
> *Thank You and Best Wishes*
> --
> *Regards*
> Garima Singh
> AcSIR-PhD Fellow
> Biotechnology Division
> CSIR-CIMAP
> Lucknow
> garimabioinfo.gmail.com
>
>
>
>
> *INDIA* Please don't print this e-mail unless you really need to. Be
> Green !
>
> On Sat, May 13, 2017 at 12:30 AM, <amber-request.ambermd.org> wrote:
>
>> Send AMBER mailing list submissions to
>>         amber.ambermd.org
>>
>> To subscribe or unsubscribe via the World Wide Web, visit
>>         http://lists.ambermd.org/mailman/listinfo/amber
>> or, via email, send a message with subject or body 'help' to
>>         amber-request.ambermd.org
>>
>> You can reach the person managing the list at
>>         amber-owner.ambermd.org
>>
>> When replying, please edit your Subject line so it is more specific
>> than "Re: Contents of AMBER digest..."
>>
>>
>> AMBER Mailing List Digest
>>
>> Today's Topics:
>>
>>    1. Re: <Na 1> Could not find vdW (or other) parameters for type:
>>       Na (David A Case)
>>    2. Re: <Na 1> Could not find vdW (or other) parameters for type:
>>       Na (Thakur, Abhishek)
>>    3. Re: Tip3p water box size for two different systems.
>>       (Elvis  Martis)
>>    4. Fwd: Problem in splitting mdcrd file with cpptraj
>>       (Manjula Saravanan)
>>    5. Re: Tip3p water box size for two different systems.
>>       (Saman Yousuf ali)
>>    6. Re: Tip3p water box size for two different systems.
>>       (Elvis  Martis)
>>    7. Re: Tip3p water box size for two different systems. (Bill Ross)
>>    8. How to use Amber in HPC (Garima Singh)
>>    9. Re: How to use Amber in HPC (Elvis  Martis)
>>   10. Re: <Na 1> Could not find vdW (or other) parameters for type:
>>       Na (David A Case)
>>   11. EEL and VDW Notification on minimization with sander/pmemd
>>       (Charles Mariasoosai)
>>
>>
>> ----------------------------------------------------------------------
>>
>> Message: 1
>> Date: Thu, 11 May 2017 15:02:00 -0400
>> From: David A Case <david.case.rutgers.edu>
>> Subject: Re: [AMBER] <Na 1> Could not find vdW (or other) parameters
>>         for type: Na
>> To: AMBER Mailing List <amber.ambermd.org>
>> Message-ID: <20170511190200.spq3psgfgfqql6fj.scarletmail.rutgers.edu>
>> Content-Type: text/plain; charset=us-ascii
>>
>> On Thu, May 11, 2017, Thakur, Abhishek wrote:
>> >
>> >
>> > I have two sodium and one chlorine ions positioned at a specific
>> > position in my complex structure.
>> >
>> > So for this complex when I am trying to make prmtop and inpcrd file I am
>> > getting an error for my sodium ions.
>> >
>> >
>> > For atom: .R<Na 600>.A<Na 1> Could not find vdW (or other) parameters
>> > for type: Na
>>
>> You should tell us what commands you gave to tleap, that is, which
>> parameters
>> (usually via leaprc files) you loaded.
>>
>> However, the correct atom and residue name for sodium ions is "NA" (for
>> both
>> the atom and the residue).  This is the PDB standard, which we try to
>> follow.  For backwards compatibility, I think tleap still recognizes
>> "Na+",
>> but that is an Amber-ism and should be discouraged.
>>
>> The correct atom/residue name for chloride is "CL".  There is not enough
>> information in your email to determine how that is being processed.  You
>> can always use the "desc" command in tleap to see what residues are
>> loaded.
>>
>> ....hope this helps....dac
>>
>>
>>
>>
>> ------------------------------
>>
>> Message: 2
>> Date: Thu, 11 May 2017 21:37:54 +0000
>> From: "Thakur, Abhishek" <axt651.miami.edu>
>> Subject: Re: [AMBER] <Na 1> Could not find vdW (or other) parameters
>>         for type: Na
>> To: AMBER Mailing List <amber.ambermd.org>, "david.case.rutgers.edu"
>>         <david.case.rutgers.edu>
>> Message-ID:
>>         <MWHPR07MB2814EC37B7BD9F42125481F09EED0.MWHPR07MB2814.namprd
>> 07.prod.outlook.com>
>>
>> Content-Type: text/plain; charset="us-ascii"
>>
>> Hi Dr. Case,
>>
>>
>> I have been doing
>>
>> tleap -s -f leaprc.ff14SB.ORIG
>> source leaprc.gaff
>> loadamberparams UNK.frcmod
>> loadoff UNK.lib
>> Na = loadmol2 Na.mol2
>> Cl = loadmol2 Cl.mol2
>> R_config = loadpdb C8_2.pdb
>> solvateBox R_config TIP3PBOX 10
>> charge R_config
>> addIons R_config Cl- 2
>> loadAmberParams frcmod.ionsjc_tip3p
>> saveamberparm R_config C8.prmtop C8.inpcrd
>> savepdb R_config complex.pdb
>> quit
>>
>>
>> ________________________________
>> From: David A Case <david.case.rutgers.edu>
>> Sent: Thursday, May 11, 2017 8:02:00 AM
>> To: AMBER Mailing List
>> Subject: Re: [AMBER] <Na 1> Could not find vdW (or other) parameters for
>> type: Na
>>
>> On Thu, May 11, 2017, Thakur, Abhishek wrote:
>> >
>> >
>> > I have two sodium and one chlorine ions positioned at a specific
>> > position in my complex structure.
>> >
>> > So for this complex when I am trying to make prmtop and inpcrd file I am
>> > getting an error for my sodium ions.
>> >
>> >
>> > For atom: .R<Na 600>.A<Na 1> Could not find vdW (or other) parameters
>> > for type: Na
>>
>> You should tell us what commands you gave to tleap, that is, which
>> parameters
>> (usually via leaprc files) you loaded.
>>
>> However, the correct atom and residue name for sodium ions is "NA" (for
>> both
>> the atom and the residue).  This is the PDB standard, which we try to
>> follow.  For backwards compatibility, I think tleap still recognizes
>> "Na+",
>> but that is an Amber-ism and should be discouraged.
>>
>> The correct atom/residue name for chloride is "CL".  There is not enough
>> information in your email to determine how that is being processed.  You
>> can always use the "desc" command in tleap to see what residues are
>> loaded.
>>
>> ....hope this helps....dac
>>
>>
>> _______________________________________________
>> AMBER mailing list
>> AMBER.ambermd.org
>> https://urldefense.proofpoint.com/v2/url?u=http-3A__lists.am
>> bermd.org_mailman_listinfo_amber&d=DwICAg&c=y2w-uYmhgFWijp_I
>> QN0DhA&r=0Hah93XWYYBgmROOVcaccg&m=nKxpXK4_KFVej2ezr8KcHwKSqr
>> 8tIcHT_B3HB1orZtA&s=5YMX75rqQOg5Rs2aVAT-Xr6iJsP0XKQoqXDxhjj3x3Y&e=
>>
>>
>> ------------------------------
>>
>> Message: 3
>> Date: Fri, 12 May 2017 05:18:59 +0000
>> From: "Elvis  Martis" <elvis.martis.bcp.edu.in>
>> Subject: Re: [AMBER] Tip3p water box size for two different systems.
>> To: Saman Yousuf ali <saman.yousufali64.yahoo.com>, AMBER Mailing List
>>         <amber.ambermd.org>
>> Message-ID:
>>         <MAXPR01MB0218C03DD70632714822818CA3E20.MAXPR01MB0218.INDPRD
>> 01.PROD.OUTLOOK.COM>
>>
>> Content-Type: text/plain; charset="utf-8"
>>
>> Hi,
>> Since the proteins will be bigger, the box size will automatically be
>> bigger if you use solvation shell method (using buffer).
>> However, I don't see a need why you must keep the box size same.
>>
>> ? ? Best Regards
>>
>>
>>
>> Elvis Martis
>> Ph.D. Student (Computational Chemistry)
>> ?at?Bombay College of Pharmacy
>>
>>
>> A??Kalina, Santacruz [E], Mumbai 400098, INDIA
>> W?www.elvismartis.in
>> Skype.?adrian_elvis12
>>
>>
>>
>>
>> -----Original Message-----
>> From: Saman Yousuf ali [mailto:saman.yousufali64.yahoo.com]
>> Sent: Thursday, May 11, 2017 8:27 PM
>> To: amber.ambermd.org
>> Subject: [AMBER] Tip3p water box size for two different systems.
>>
>> Dear All,
>> I am interested to simulate complex protein system in dimeric and
>> monomeric form separately. Residues in case of monomeric system is 1-268
>> including one Ligand and cofactor. Dimeric system is double in size. My
>> question is for solvation of each systems tip3p water size should be same
>> for both? or dimeric system box size must be bigger in size as compared to
>> monomer?
>>
>> Thanks
>>
>>
>>
>>
>> ?
>> ?
>>
>> _______________________________________________
>> AMBER mailing list
>> AMBER.ambermd.org
>> http://lists.ambermd.org/mailman/listinfo/amber
>>
>> ------------------------------
>>
>> Message: 4
>> Date: Fri, 12 May 2017 10:50:31 +0530
>> From: Manjula Saravanan <manjusimba.gmail.com>
>> Subject: [AMBER] Fwd: Problem in splitting mdcrd file with cpptraj
>> To: amber.ambermd.org
>> Message-ID:
>>         <CANtcf8AmC6dK0EaN9zMWhvZV8UZ-s_dKL9Nf_3YW62eZsDq26g.mail.gm
>> ail.com>
>> Content-Type: text/plain; charset="UTF-8"
>>
>> *With Best Regards*
>> *S. Manjula*
>> *Research Scholar*
>> *Laboratory of Biocrystallography and Computational Molecular Biology*
>> *Department of Physics*
>> *Periyar University*
>> *Salem-11*
>> *Tamilnadu*
>>
>>
>>
>> Dear Sir/Madam,
>>                 I am trying to split my mdcrd file which contains 1580
>> frames. I want only 50 frames starting from 1159-1209 for the normal mode
>> calculation. my input file is,
>>
>> t
>>
>>
>> *rajin prod3.mdcrd 1159 1209 1 trajout prod30ns_50frames1.mdcrd*
>> But it shows some error in the output as follows,
>>
>>
>>
>>
>>
>>
>>
>>
>>
>>
>>
>>
>>
>> *Error: start 1159 > #Frames (141), no frames will be processed.Error:
>> Could not set up input trajectory 'prod3.mdcrd'.    1 errors encountered
>> reading input.CPPTRAJ: Trajectory Analysis. V14.25    ___  ___  ___
>> ___     | \/ | \/ | \/ |     _|_/\_|_/\_|_/\_|_    Reading
>> 'com_solv.prmtop' as Amber TopologyINPUT: Reading Input from file
>> cpptraj.in <http://cpptraj.in>  [trajin prod3.mdcrd 1159 1209 50 ]
>> Reading 'prod3.mdcrd' as Amber TrajectoryTIME: Total execution time:
>> 0.3070
>> seconds.*
>>
>> Kindly help me to solve this problem.
>>
>> *With Best Regards*
>> *S. Manjula*
>> *Research Scholar*
>> *Laboratory of Biocrystallography and Computational Molecular Biology*
>> *Department of Physics*
>> *Periyar University*
>> *Salem-11*
>> *Tamilnadu*
>>
>>
>> ------------------------------
>>
>> Message: 5
>> Date: Fri, 12 May 2017 05:30:43 +0000 (UTC)
>> From: Saman Yousuf ali <saman.yousufali64.yahoo.com>
>> Subject: Re: [AMBER] Tip3p water box size for two different systems.
>> To: Elvis Martis <elvis.martis.bcp.edu.in>,     AMBER Mailing List
>>         <amber.ambermd.org>
>> Message-ID: <212545802.10940389.1494567043539.mail.yahoo.com>
>> Content-Type: text/plain; charset=UTF-8
>>
>> Dear Martis,Thanks for response. I do not want to use same box size, I
>> understand that as system size increase water box size should be bigger.? I
>> am just asking about box size idea for my system. like if I generate 8
>> angstrom tip3p box around my monomeric system then what is the ideal box
>> size for dimer? I hope you get my point.
>>
>> Thanks
>> ?
>>
>>
>>     On Friday, May 12, 2017 10:19 AM, Elvis Martis <
>> elvis.martis.bcp.edu.in> wrote:
>>
>>
>>  Hi,
>> Since the proteins will be bigger, the box size will automatically be
>> bigger if you use solvation shell method (using buffer).
>> However, I don't see a need why you must keep the box size same.
>>
>> ? ? Best Regards
>>
>>
>>
>> Elvis Martis
>> Ph.D. Student (Computational Chemistry)
>> ?at?Bombay College of Pharmacy
>>
>>
>> A??Kalina, Santacruz [E], Mumbai 400098, INDIA
>> W?www.elvismartis.in
>> Skype.?adrian_elvis12
>>
>>
>>
>>
>> -----Original Message-----
>> From: Saman Yousuf ali [mailto:saman.yousufali64.yahoo.com]
>> Sent: Thursday, May 11, 2017 8:27 PM
>> To: amber.ambermd.org
>> Subject: [AMBER] Tip3p water box size for two different systems.
>>
>> Dear All,
>> I am interested to simulate complex protein system in dimeric and
>> monomeric form separately. Residues in case of monomeric system is 1-268
>> including one Ligand and cofactor. Dimeric system is double in size. My
>> question is for solvation of each systems tip3p water size should be same
>> for both? or dimeric system box size must be bigger in size as compared to
>> monomer?
>>
>> Thanks
>>
>>
>>
>>
>> ?
>> ?
>>
>> _______________________________________________
>> AMBER mailing list
>> AMBER.ambermd.org
>> http://lists.ambermd.org/mailman/listinfo/amber
>>
>>
>>
>>
>> ------------------------------
>>
>> Message: 6
>> Date: Fri, 12 May 2017 05:42:34 +0000
>> From: "Elvis  Martis" <elvis.martis.bcp.edu.in>
>> Subject: Re: [AMBER] Tip3p water box size for two different systems.
>> To: Saman Yousuf ali <saman.yousufali64.yahoo.com>, AMBER Mailing List
>>         <amber.ambermd.org>
>> Message-ID:
>>         <MAXPR01MB0218A4C8C7BCF1375A8349BFA3E20.MAXPR01MB0218.INDPRD
>> 01.PROD.OUTLOOK.COM>
>>
>> Content-Type: text/plain; charset="utf-8"
>>
>> Hi,
>> There is nothing idea here.
>> You can use 8 angstrom buffer for both your dimer and your monomer and
>> there should be no problem.
>>
>>     Best Regards
>>
>>
>>
>> Elvis Martis
>> Ph.D. Student (Computational Chemistry)
>>  at Bombay College of Pharmacy
>>
>>
>>
>> A  Kalina, Santacruz [E], Mumbai 400098, INDIA
>> W www.elvismartis.in<https://webapp.wisestamp.com/www.elvismartis.in>
>>
>> Skype. adrian_elvis12<https://webapp.wisestamp.com/>
>>
>>
>>
>>
>>
>> From: Saman Yousuf ali [mailto:saman.yousufali64.yahoo.com]
>> Sent: Friday, May 12, 2017 11:01 AM
>> To: Elvis Martis <elvis.martis.bcp.edu.in>; AMBER Mailing List <
>> amber.ambermd.org>
>> Subject: Re: [AMBER] Tip3p water box size for two different systems.
>>
>> Dear Martis,
>> Thanks for response. I do not want to use same box size, I understand
>> that as system size increase water box size should be bigger.  I am just
>> asking about box size idea for my system. like if I generate 8 angstrom
>> tip3p box around my monomeric system then what is the ideal box size for
>> dimer? I hope you get my point.
>>
>> Thanks
>>
>>
>>
>> On Friday, May 12, 2017 10:19 AM, Elvis Martis <elvis.martis.bcp.edu.in
>> <mailto:elvis.martis.bcp.edu.in>> wrote:
>>
>> Hi,
>> Since the proteins will be bigger, the box size will automatically be
>> bigger if you use solvation shell method (using buffer).
>> However, I don't see a need why you must keep the box size same.
>>
>>     Best Regards
>>
>>
>>
>> Elvis Martis
>> Ph.D. Student (Computational Chemistry)
>>  at Bombay College of Pharmacy
>>
>>
>> A  Kalina, Santacruz [E], Mumbai 400098, INDIA
>> W www.elvismartis.in<http://www.elvismartis.in>
>> Skype. adrian_elvis12
>>
>>
>>
>> -----Original Message-----
>> From: Saman Yousuf ali [mailto:saman.yousufali64.yahoo.com<mailto:
>> saman.yousufali64.yahoo.com>]
>> Sent: Thursday, May 11, 2017 8:27 PM
>> To: amber.ambermd.org<mailto:amber.ambermd.org>
>> Subject: [AMBER] Tip3p water box size for two different systems.
>>
>> Dear All,
>> I am interested to simulate complex protein system in dimeric and
>> monomeric form separately. Residues in case of monomeric system is 1-268
>> including one Ligand and cofactor. Dimeric system is double in size. My
>> question is for solvation of each systems tip3p water size should be same
>> for both? or dimeric system box size must be bigger in size as compared to
>> monomer?
>>
>> Thanks
>>
>>
>>
>>
>>
>>
>>
>>
>> _______________________________________________
>> AMBER mailing list
>> AMBER.ambermd.org<mailto:AMBER.ambermd.org>
>> http://lists.ambermd.org/mailman/listinfo/amber
>>
>>
>>
>> ------------------------------
>>
>> Message: 7
>> Date: Thu, 11 May 2017 22:52:06 -0700
>> From: Bill Ross <ross.cgl.ucsf.edu>
>> Subject: Re: [AMBER] Tip3p water box size for two different systems.
>> To: AMBER Mailing List <amber.ambermd.org>
>> Message-ID: <f8a144e0-0ff7-599e-a903-ca92b990136b.cgl.ucsf.edu>
>> Content-Type: text/plain; charset=windows-1252; format=flowed
>>
>> 8 Angstroms seems small in both cases. I would consider 10, since the
>> system will shrink on equilibration, as inititial vdw voids go away.
>>
>> Bil;
>>
>>
>> On 5/11/17 10:42 PM, Elvis Martis wrote:
>> > Hi,
>> > There is nothing idea here.
>> > You can use 8 angstrom buffer for both your dimer and your monomer and
>> there should be no problem.
>> >
>> >      Best Regards
>> >
>> >
>> >
>> > Elvis Martis
>> > Ph.D. Student (Computational Chemistry)
>> >   at Bombay College of Pharmacy
>> >
>> >
>> >
>> > A  Kalina, Santacruz [E], Mumbai 400098, INDIA
>> > W www.elvismartis.in<https://webapp.wisestamp.com/www.elvismartis.in>
>> >
>> > Skype. adrian_elvis12<https://webapp.wisestamp.com/>
>> >
>> >
>> >
>> >
>> >
>> > From: Saman Yousuf ali [mailto:saman.yousufali64.yahoo.com]
>> > Sent: Friday, May 12, 2017 11:01 AM
>> > To: Elvis Martis <elvis.martis.bcp.edu.in>; AMBER Mailing List <
>> amber.ambermd.org>
>> > Subject: Re: [AMBER] Tip3p water box size for two different systems.
>> >
>> > Dear Martis,
>> > Thanks for response. I do not want to use same box size, I understand
>> that as system size increase water box size should be bigger.  I am just
>> asking about box size idea for my system. like if I generate 8 angstrom
>> tip3p box around my monomeric system then what is the ideal box size for
>> dimer? I hope you get my point.
>> >
>> > Thanks
>> >
>> >
>> >
>> > On Friday, May 12, 2017 10:19 AM, Elvis Martis <elvis.martis.bcp.edu.in
>> <mailto:elvis.martis.bcp.edu.in>> wrote:
>> >
>> > Hi,
>> > Since the proteins will be bigger, the box size will automatically be
>> bigger if you use solvation shell method (using buffer).
>> > However, I don't see a need why you must keep the box size same.
>> >
>> >      Best Regards
>> >
>> >
>> >
>> > Elvis Martis
>> > Ph.D. Student (Computational Chemistry)
>> >   at Bombay College of Pharmacy
>> >
>> >
>> > A  Kalina, Santacruz [E], Mumbai 400098, INDIA
>> > W www.elvismartis.in<http://www.elvismartis.in>
>> > Skype. adrian_elvis12
>> >
>> >
>> >
>> > -----Original Message-----
>> > From: Saman Yousuf ali [mailto:saman.yousufali64.yahoo.com<mailto:
>> saman.yousufali64.yahoo.com>]
>> > Sent: Thursday, May 11, 2017 8:27 PM
>> > To: amber.ambermd.org<mailto:amber.ambermd.org>
>> > Subject: [AMBER] Tip3p water box size for two different systems.
>> >
>> > Dear All,
>> > I am interested to simulate complex protein system in dimeric and
>> monomeric form separately. Residues in case of monomeric system is 1-268
>> including one Ligand and cofactor. Dimeric system is double in size. My
>> question is for solvation of each systems tip3p water size should be same
>> for both? or dimeric system box size must be bigger in size as compared to
>> monomer?
>> >
>> > Thanks
>> >
>> >
>> >
>> >
>> >
>> >
>> >
>> >
>> > _______________________________________________
>> > AMBER mailing list
>> > AMBER.ambermd.org<mailto:AMBER.ambermd.org>
>> > http://lists.ambermd.org/mailman/listinfo/amber
>> >
>> >
>> > _______________________________________________
>> > AMBER mailing list
>> > AMBER.ambermd.org
>> > http://lists.ambermd.org/mailman/listinfo/amber
>>
>>
>>
>>
>> ------------------------------
>>
>> Message: 8
>> Date: Fri, 12 May 2017 16:23:49 +0530
>> From: Garima Singh <garimabioinfo.gmail.com>
>> Subject: [AMBER] How to use Amber in HPC
>> To: amber.ambermd.org
>> Message-ID:
>>         <CAD=mwY1K1a0GkNUpTekGnmM2NQ1WtEfOqjf5uYE2Lt+ZaZWt6g.mail.gm
>> ail.com>
>> Content-Type: text/plain; charset="UTF-8"
>>
>> Dear Amber users,
>>
>>
>> I am using AMBER 14 in my system having processor* Intel? Xeon(R) CPU
>> E5-1607 v3 . 3.10GHz* *? 4* . It takes a lot time to calculating the
>> output.I want to run my  Amber MD calculation in HPC. How to perform MD
>> calculation using AMBER 14 in HPC .Which script file i need?
>>
>>  Kindly provide your valuable suggestion
>>
>> Thanks
>> *Regards*
>> Garima Singh
>> AcSIR-PhD Fellow
>> Central Institute Of Medicinal And Aromatic Plant
>> CSIR-CIMAP
>> Lucknow
>> garimabioinfo.gmail.com
>>
>>
>>
>>
>> *INDIA* Please don't print this e-mail unless you really need to. Be
>> Green !
>>
>>
>> ------------------------------
>>
>> Message: 9
>> Date: Fri, 12 May 2017 11:40:31 +0000
>> From: "Elvis  Martis" <elvis.martis.bcp.edu.in>
>> Subject: Re: [AMBER] How to use Amber in HPC
>> To: AMBER Mailing List <amber.ambermd.org>
>> Message-ID:
>>         <MAXPR01MB0218ACE31AD2FAAF62ECFDF5A3E20.MAXPR01MB0218.INDPRD
>> 01.PROD.OUTLOOK.COM>
>>
>> Content-Type: text/plain; charset="utf-8"
>>
>> Hi
>> You will need a pbs or torque script to submit any kind of jobs on the
>> HPC.
>> The best would be to consult the system admin for the HPC
>> A typical pbs script will look like this, you must edit it to suit your
>> system and your needs
>>
>> #!/bin/bash
>> #PBS -l nodes=2, ppn=2
>> #PBS -l walltime=50:00:00
>> #PBS -j oe
>> #PBS -q normal
>> #PBS -N <JOB NAME>
>> #PBS -l pmem=2048MB
>> #PBS -l vmem=2048MB
>>  cat $PBS_NODEFILE
>> cd <WORK DIRECTORY>
>>
>> set mpich_run =  "XYZ/ mpirun"  >>> consult system admin
>> set sander.MPI (pmemd.MPI) = "$AMBERHOME/bin/sander.MPI(or pmemd.MPI)"
>> >> pointer for sander(or pmemd)
>> $mpich_run -machinefile $PBS_NODEFILE -np `wc -l < $PBS_NODEFILE`
>> $mpich_run -np $NSLOTS $sander.MPI (or $pmemd.MPI) -O -i INFILE -c
>> INPUT_CORDINATE -o outfile -r output_coordinate -x trajectory_file   >>>
>> sander command will remain same
>>
>>
>> ? ? Best Regards
>>
>>
>>
>> Elvis Martis
>> Ph.D. Student (Computational Chemistry)
>> ?at?Bombay College of Pharmacy
>>
>>
>> A??Kalina, Santacruz [E], Mumbai 400098, INDIA
>> W?www.elvismartis.in
>> Skype.?adrian_elvis12
>>
>>
>>
>>
>> -----Original Message-----
>> From: Garima Singh [mailto:garimabioinfo.gmail.com]
>> Sent: Friday, May 12, 2017 4:24 PM
>> To: amber.ambermd.org
>> Subject: [AMBER] How to use Amber in HPC
>>
>> Dear Amber users,
>>
>>
>> I am using AMBER 14 in my system having processor* Intel? Xeon(R) CPU
>> E5-1607 v3 . 3.10GHz* *? 4* . It takes a lot time to calculating the
>> output.I want to run my  Amber MD calculation in HPC. How to perform MD
>> calculation using AMBER 14 in HPC .Which script file i need?
>>
>>  Kindly provide your valuable suggestion
>>
>> Thanks
>> *Regards*
>> Garima Singh
>> AcSIR-PhD Fellow
>> Central Institute Of Medicinal And Aromatic Plant CSIR-CIMAP Lucknow
>> garimabioinfo.gmail.com
>>
>>
>>
>>
>> *INDIA* Please don't print this e-mail unless you really need to. Be
>> Green !
>> _______________________________________________
>> AMBER mailing list
>> AMBER.ambermd.org
>> http://lists.ambermd.org/mailman/listinfo/amber
>>
>> ------------------------------
>>
>> Message: 10
>> Date: Fri, 12 May 2017 08:33:34 -0400
>> From: David A Case <david.case.rutgers.edu>
>> Subject: Re: [AMBER] <Na 1> Could not find vdW (or other) parameters
>>         for type: Na
>> To: AMBER Mailing List <amber.ambermd.org>
>> Message-ID: <20170512123334.s45ul3lt6wlucrpg.scarletmail.rutgers.edu>
>> Content-Type: text/plain; charset=us-ascii
>>
>> On Thu, May 11, 2017, Thakur, Abhishek wrote:
>> >
>> > I have been doing
>> >
>> > tleap -s -f leaprc.ff14SB.ORIG
>> > source leaprc.gaff
>> > loadamberparams UNK.frcmod
>> > loadoff UNK.lib
>> > Na = loadmol2 Na.mol2
>> > Cl = loadmol2 Cl.mol2
>> > R_config = loadpdb C8_2.pdb
>> > solvateBox R_config TIP3PBOX 10
>> > charge R_config
>> > addIons R_config Cl- 2
>> > loadAmberParams frcmod.ionsjc_tip3p
>> > saveamberparm R_config C8.prmtop C8.inpcrd
>> > savepdb R_config complex.pdb
>> > quit
>>
>> OK: you are rolling your own commands, and are pretty much on your own
>> to see what is going wrong.  Consider using standard leaprc files (e.g.
>> leaprc.protein.ff14SB, leaprc.water.tip3p).
>>
>> I note that you called chloride "Cl" in the loadmol2 command, but called
>> it "Cl-" in the addIons command.  Look carefully at the leap.log file to
>> see exactly what is going on.
>>
>> Here's my best guess: you get the error for "Na" because the Amber
>> libraries
>> recognize "NA" and "Na+" (for backward compatibility), but don't have any
>> entries for "Na".  There was no error for chloride because of the above
>> typo
>> in the addIons command.  Easiest fix is probably to edit your pdb file
>> and use "NA" and "CL" for sodium and chloride ions.
>>
>> ....dac
>>
>>
>>
>>
>> ------------------------------
>>
>> Message: 11
>> Date: Fri, 12 May 2017 22:27:53 +0530
>> From: Charles Mariasoosai <charlesmariasoosai51.gmail.com>
>> Subject: [AMBER] EEL and VDW Notification on minimization with
>>         sander/pmemd
>> To: amber.ambermd.org
>> Message-ID:
>>         <CABu9AX134b3DdUPKPTUCddRYO-AC0YcjJF1Ynv2qed_i7Bo=aw.mail.gm
>> ail.com>
>> Content-Type: text/plain; charset="UTF-8"
>>
>> Am new to amber.
>> i have generated parameters for non standard(modified: covalently attached
>> with co-factor ) amino acid and included in my library.
>> i have successfully generated prmtop and inpcrd files.
>> While running minimisation am getting the folwing notification in out file
>> and my minimisation is not proceeding forward?
>>
>>
>>
>>
>>
>>
>>
>> *| Note: 1-4 EEL scale factors are being read from the topology file.|
>> Note: 1-4 VDW scale factors are being read from the topology file. Found a
>> non-zero 10-12 coefficient, but source  was not compiled with
>> -DHAS_10_12. If you are using a pre-1994 force field, you  will need to
>> re-compile with this flag.*
>>
>>
>> how i should solve this ?
>> and am getting segmentaion fault in terminal.
>>
>>
>>
>> --
>>
>> *-Regards-*
>>
>> *?. ???? ?????? ???????(M.Ramya Chandar Charles*)
>> Research Scholar
>> c/o Dr. S. Mohane Coumar
>> Centre for Bioinformatics
>> Pondicherry university
>> Mob: +91-9283684619
>>
>>
>> ------------------------------
>>
>> _______________________________________________
>> AMBER mailing list
>> AMBER.ambermd.org
>> http://lists.ambermd.org/mailman/listinfo/amber
>>
>>
>> End of AMBER Digest, Vol 1932, Issue 1
>> **************************************
>>
>
>
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