20.109:TAP-tags: Difference between revisions

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(New page: ==New Protein Engineering Module for F08== Point of departure is to ask if tags are actually neutral wrt protein function ===Rough sketch of labs=== *Part 1: TAP tag **non-essential SAGA ...)
 
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**non-essential SAGA subunits (essential likely in many complexes so purif profile complex + tag has many consequences)
**non-essential SAGA subunits (essential likely in many complexes so purif profile complex + tag has many consequences)
**unknown ORFs changed during microarray of SAGA del or mtRNT1
**unknown ORFs changed during microarray of SAGA del or mtRNT1
1-1 Design primers<br>
***1-1 Design primers<br>
1-2 PCR<br>
***1-2 PCR<br>
1-3 Transform<br>
***1-3 Transform<br>
1-4 Confirm integration by colony PCR <br>
***1-4 Confirm integration by colony PCR <br>
**Alternatively, could just give students tagged version.
**Alternatively, could just give students tagged version.
*Part 2: Western
*Part 2: Western
** need + TAP control
** need + TAP control
** use Sigma Ab to protA (PAP P-2026, anti-ProtA)
** use Sigma Ab to protA ([http://www.sigmaaldrich.com/catalog/search/ProductDetail/SIGMA/P3775 anti-ProtA raised in rabbit] or if need to detect tag when protA has been cleaved can use [http://www.openbiosystems.com/ProductLiterature.aspx?AliasPath=/antibodies/catalog/tag&CatalogNumber=CAB1001 OpenBiosystems Ab])
** 1.5 ml ON culture, vortex 3X30' with glass beads and add 100 ul LB from [http://www.ncbi.nlm.nih.gov/sites/entrez Methods (2001) 24:218]
** 1.5 ml ON culture, vortex 3X30' with glass beads and add 100 ul LB from [http://www.ncbi.nlm.nih.gov/sites/entrez Methods (2001) 24:218] [http://library.mit.edu/item/000594799 barton link]
*Part 3: Phenotypes
*Part 3: Phenotypes
** compare parental, K/O, TAP-tagged
** compare parental, K/O, TAP-tagged
** examine GAL, Spt (his4-917d), TS, CS
** examine GAL, Spt (his4-917d), TS, CS
*Part 4: Array
*Part 4: [http://www.chem.agilent.com/scripts/pds.asp?lPage=37069 Array]
** compare parental to TAP-tagged
** compare parental to TAP-tagged
===Could also include===
*Could also include
Mass Spec analysis description/tour/lab? <br>
**Mass Spec analysis description/tour/lab? <br>
Tour of protein purif facilty
**Tour of protein purif facility
 
===Experimental Details===
====Bacteria====
* FB2305 = NB 311
**MC1066+pBS1539 (AmpR+URA3-Kl, TAP tag)
*FB2306 = NB312
**MC1066+pBS1479(AmpR+TRP1-Kl, TAP tag)
** ref for seq of TRP1 from Kluyveromyces lactis [http://www.ncbi.nlm.nih.gov/pubmed/2538971 here]
** NCBI link for seq of TRP1 from Kluyveromyces lactis [http://www.ncbi.nlm.nih.gov/sites/entrez?db=nuccore&cmd=search&term=trp1%20k.%20lactis here]
[[Image:TAPplasmids.png|thumb|left|600px| from Methods 2001 article[http://www.sciencedirect.com/science?_ob=ArticleURL&_udi=B6WN5-456JRHJ-17&_user=10&_rdoc=1&_fmt=&_orig=search&_sort=d&view=c&_acct=C000050221&_version=1&_urlVersion=0&_userid=10&md5=53bcb4f821b860dce449e6105fb83081]]]
*NB318
**XL1-bl+pBS1479 (Lisa's prep of plasmid which does give PCR product for TAP-TRP, freshly transformed)
====Yeast====
*<b>FY631 = Parental for TAP tagging</b> = NY411
**MATa, his4-917d, lys2-173R2, leu2d1, ura3-52, trp1d63 
*FY2714 = NY412
**MATa, <b>HA-SPT3-TAP::TRP1</b>, his4-917d, lys2-173R2, ura3D0 or -52, leu2D1 or D0, trp1D63
*FY2031 = NY413
**MATa, <b>HA-SPT7-TAP::TRP1</b>, his4-917d, lys2-173R2, ura3D0, leu2D1, trp1D63
*FY2305 = NY414
**MATa, <b>SPT10-TAP::TRP1</b> trp1D63 his3D200 leu2D1 ura3-52 lys2-128d
**<b> not his4-912d</b>
*FY2306 = NY415
**MATa, <b>SPT21-TAP::TRP1</b> trp1D63 his3D200 leu2D1 ura3-52 lys2-128d
**<b> not his4-912d</b>
====Primers for C-terminal fusions====
=====General format for=====
*Upstream primer: 40nt then TCC ATG GAA AAG AGA AG
*Downstream primer: 40nt then TAC GAC TCA CTA TAG GG
=====Relevant sequence files=====
# sequence of TAP tag only [[Media:Seq TAPtag.rtf| here]]
# sequence of pBS1479 [[Media:Seq pBS1479 TAP+TRP.rtf| here]]
[[Image:Tag structure.gif|thumb|left|600 px| from [http://www-db.embl-heidelberg.de/jss/servlet/de.embl.bk.wwwTools.GroupLeftEMBL/ExternalInfo/seraphin/TAPdescription.html]]]
[[Image:Tagging.gif|thumb|400 px|left| from [http://www-db.embl-heidelberg.de/jss/servlet/de.embl.bk.wwwTools.GroupLeftEMBL/ExternalInfo/seraphin/TAPtagging.html]]]
=====Needed primers=====
 
{| border= "1"
! needed to
! forward primer (5' to 3')
! reverse primer (5' to 3'
|--
| add TAP TRP to C-term of [http://db.yeastgenome.org/cgi-bin/locus.pl?locus=YER067W unknown 8]
| '''NO222'''<br>GGT ATT TGT CGA TTA CAA AAC ACA TCC TGT AGG CGC AAA TTC CAT GGA AAA GAG AAG <br> 57 mer <br> Tm = 66.7<br>  landing Tm (17bases only) = 45.5
| '''NO223'''<br>
GTT AGG ATT CAG TAC TAA CAC ATT CTC TAT GAC ACA ACC TTA CGA CTC ACT ATA GGG <br> 57 mer<br> Tm = 65.0 <br> landing Tm (17bases only)= 46.1
|--
| check TAP
| '''NO224'''<br>TCC ATG GAA AAG AGA AGA TGG AAA AAG AAT TTC ATA GCC GTC TC<br> 44 mer <br> Tm = 63.6 <br> use with reverse primer from tagging PCR <br>
| '''NO225'''<br>TCA GGT TGA CTT CCC CGC GGA ATT CGC GTC TAC  <br> 33 mer <br> Tm = 67.9 <br> use with fwd primer from tagging PCR<br>expect length of TAP seq + TRP K. l seq = 554 bps (from 2147 to 2701 in pBS1479) <br>
|--
| add TAP TRP to C-term of RNT1
| '''NO226'''<br>CTC ACA AAA GAA TAA GAA AAG AAA ATT CTC AGA TAC AAG CTC CAT GGA AAA GAG AAG  <br> 57 mer <br> Tm = 63.8 <br>
| '''NO227'''<br>ATC AAT GCA AGT TCC ATC ATG GTT GTG TAA AAG GAA CGT TTA CGA CTC ACT ATA GGG  <br> 57 mer <br> Tm = 66.9 <br>
|--
| longer landing sequences
|TCC ATG GAA AAG AGA AGA TG = 20 mer fwd landing <br> Tm = 49.6 ºC
|TAC GAC TCA CTA TAG GGC GA = 20 mer rev landing <br> Tm = 54.3 ºC
|--
| Unknown 8 + longer landing sequences
| '''NO228'''<br> GT ATT TGT CGA TTA CAA AAC ACA TCC TGT AGG CGC AAA TTC CAT GGA AAA GAG AAG ATG<br> 59 mer <br> Tm = 66.5 ºC
| '''NO229'''<br> TT AGG ATT CAG TAC TAA CAC ATT CTC TAT GAC ACA ACC TTA CGA CTC ACT ATA GGG CGA <br> 59 mer <br> Tm = 66.6 ºC
|--
| RNT1 + longer landing sequences
|'''NO230'''<br> TCACAA AAGAATAAGA AAAGAAAATT CTCAGATACA AGC TCC ATG GAA AAG AGA AGA TG <br> 59 mer <br> Tm = 64.4 ºC
|'''NO231'''<br> TCA ATG CAA GTT CCA TCA TGG TTG TGT AAA AGG AAC GTT TAC GAC TCA CTA TAG GGC GA <br> 59 mer <br> Tm = 68.4 ºC
|--
| check TAP
| '''NO258''' for SPT3-TAP control<br>TTT AAA GGT GGT AGA CTC AGT TCT AAA CCA ATT ATC ATG tcc atg gaa aag aga aga tg<br> 59 mer <br> use with NO225 = reverse primer for checking TAP tag <br>expect length of TAP seq + TRP K. l seq = 554 bps (from 2147 to 2701 in pBS1479) <br> 
| '''NO259'''for SPT7-TAP control<br> AAT AGT TCA TTT AGC TTG AGC CTT CCT CGC CTT AAT CAA tcc atg gaa aag aga aga tg<br> 59 mer <br> use with NO225 = reverse primer for checking TAP tag<br>expect length of TAP seq + TRP K. l seq = 554 bps (from 2147 to 2701 in pBS1479) <br>
|--
| Check TAP with NO224
|SPT3_check_rev<br>'''NO268'''<br>ACC AGA AGG AAA CCC ATG CAC CTC CAT GAT GAA ATT ATA CAA AAA T
||SPT7_check_rev<br>'''NO269'''<br>AGC AAA TGT ATT TAA TTA AAG ATA AAA TAT TCA ACT ATT TAG CGC GCT CA
|}
 
====Genes to tag====
=====Option 1: S. cerevisiae SAGA subunits=====
{| border="1"
! Subunit 
! size,chromosome,null p-type 
|--
| colspan="2" |
|-- 
| colspan="2"| Ada subunits
|--
| colspan="2" |
|-- 
| [http://db.yeastgenome.org/cgi-bin/locus.pl?locus=ADA1 Ada1] (aka HFI1, SUP110, SRM12, GAN1)
| 1.467 kb=489 aa, Chr. XVI, viable
|-   
| [http://db.yeastgenome.org/cgi-bin/locus.pl?locus=ADA2 Ada2] (aka SWI8) 
| 1.305 kb=434aa, Chr. IV, viable
|-   
| [http://db.yeastgenome.org/cgi-bin/locus.pl?locus=ADA3 Ada3](aka NGG1, SWI7) 
| 2.109 kb=702aa, Chr. IV, viable 
|- 
| [http://db.yeastgenome.org/cgi-bin/locus.pl?locus=GCN5 Gcn5] (aka ADA4, SWI9) 
| 1.32 kb=439aa, Chr. VII, viable
|- 
| [http://db.yeastgenome.org/cgi-bin/locus.pl?locus=Ada5 Ada5] (aka SPT20)
| 1.815 kb=604aa, Chr. XV, viable
|--
| colspan="2" |
|-- 
| colspan="2"| Spt subunits
|--
| colspan="2" |
|--     
| [http://db.yeastgenome.org/cgi-bin/locus.pl?locus=spt3 Spt3] 
| 1.014 kb=337aa, Chr. IV, viable
|-   
| [http://db.yeastgenome.org/cgi-bin/locus.pl?locus=Spt7 Spt7](aka GIT2) 
| 3.999 kb=1332aa, Chr. II, viable 
|-
| [http://db.yeastgenome.org/cgi-bin/locus.pl?locus=Spt8 Spt8] 
| 1.809 kb=602aa, Chr. XII, viable
|- 
| [http://db.yeastgenome.org/cgi-bin/locus.pl?locus=SPT20 Spt20] (aka Ada5) 
| 1.815 kb=604aa, Chr. XV, viable
|--
| colspan="2" |
|-- 
| colspan="2"| TAF subunits
|--
| colspan="2" |
|--     
| [http://db.yeastgenome.org/cgi-bin/locus.pl?locus=TAF5 TAF5] (aka TAF90) 
| 2.397 kb=798aa, Chr. II, <font color = red>inviable</font color>
|-
| [http://db.yeastgenome.org/cgi-bin/locus.pl?locus=TAF6 TAF6] (aka TAF60) 
| 1.551 kb=516aa, Chr. VII, <font color = red>inviable</font color>
|- 
| [http://db.yeastgenome.org/cgi-bin/locus.pl?locus=TAF9 TAF9] (aka TAF17) 
| 0.474 kb=157aa, Chr. XIII, <font color = red>inviable</font color>
|-
| [http://db.yeastgenome.org/cgi-bin/locus.pl?locus=TAF10 TAF10] (aka TAF23, TAF25)
| 0.621 kb=206aa, Chr. IV, <font color = red>inviable</font color>
|-
| [http://db.yeastgenome.org/cgi-bin/locus.pl?locus=TAF12 TAF12](aka TAF61, TAF68)
| 1.620 kb=539aa, Chr. IV, <font color = red>inviable</font color> 
|--
| colspan="2" |
|-- 
| colspan="2"| Tra subunit
|--
| colspan="2" |
|--   
| [http://db.yeastgenome.org/cgi-bin/locus.pl?locus=TRA1 Tra1] 
| 11.235 kb=3744aa, Chr. VIII, <font color = red>inviable</font color>
|--
| colspan="2" |
|-- 
| colspan="2"| Other subunits
|--
| colspan="2" |
|--   
| [http://db.yeastgenome.org/cgi-bin/locus.pl?locus=sgf73 Sgf73] 
| 1.974 kb=657aa, Chr. VII , viable
|-
| [http://db.yeastgenome.org/cgi-bin/locus.pl?locus=sgf29 Sgf29] 
| 0.779 kb=259aa, Chr. III, viable
|-
| [http://db.yeastgenome.org/cgi-bin/locus.pl?locus=sgf11 Sgf11] 
| 0.3 kb=99aa, Chr.XVI, viable
|-
| [http://db.yeastgenome.org/cgi-bin/locus.pl?locus=ubp8 Ubp8] 
| 1.416 kb=471aa, Chr. XIII, viable
|- 
| [http://db.yeastgenome.org/cgi-bin/locus.pl?locus=Sus1 Sus1] 
| gene with intron, Chr. II, viable 
|}
=====Option 2: Unknown ORFs from SGF73/sgf73 array=====
{| border="1"
! Unknown
! ORF 
! SGF73 green signal
! sgf73 red signal
! log2 (green/red) 
|--
|1
|[http://db.yeastgenome.org/cgi-bin/locus.pl?locus=YHR033W YHR033W]
|38938 and 69586
|285 and 570
|7.1 and 6.9
|--
|2
|[http://db.yeastgenome.org/cgi-bin/locus.pl?locus=YOR302W YOR302W]
|3374 and 6054
|49 and 167
|6.1 and 5.2
|--
|3
|[http://db.yeastgenome.org/cgi-bin/locus.pl?locus=YJR097W YJR097W]
|524 and 1052
|13 and 28
|5.3 and 5.2
|--
|4
|[http://db.yeastgenome.org/cgi-bin/locus.pl?locus=YBL028C YBL028C]
|1146 and 2706
|32 and 323
|5.2 and 3.1
|--
|5
|[http://db.yeastgenome.org/cgi-bin/locus.pl?locus=YDR034W-B YDR034W-B]
|17290
|447
|5.3
|--
|6
|[http://db.yeastgenome.org/cgi-bin/locus.pl?locus=YGR067C YGR067C]
|12025
|320
|5.2
|--
|7
|[http://db.yeastgenome.org/cgi-bin/locus.pl?locus=YKL037W YKL037W]
|8340
|282
|4.9
|--
|8
|[http://db.yeastgenome.org/cgi-bin/locus.pl?locus=YER067W YER067W]
| 6296 and 12450
| 82556 and 81036
| -3.7 and -2.7
|}

Latest revision as of 12:17, 3 September 2008

New Protein Engineering Module for F08

Point of departure is to ask if tags are actually neutral wrt protein function

Rough sketch of labs

  • Part 1: TAP tag
    • non-essential SAGA subunits (essential likely in many complexes so purif profile complex + tag has many consequences)
    • unknown ORFs changed during microarray of SAGA del or mtRNT1
      • 1-1 Design primers
      • 1-2 PCR
      • 1-3 Transform
      • 1-4 Confirm integration by colony PCR
    • Alternatively, could just give students tagged version.
  • Part 2: Western
  • Part 3: Phenotypes
    • compare parental, K/O, TAP-tagged
    • examine GAL, Spt (his4-917d), TS, CS
  • Part 4: Array
    • compare parental to TAP-tagged
  • Could also include
    • Mass Spec analysis description/tour/lab?
    • Tour of protein purif facility

Experimental Details

Bacteria

  • FB2305 = NB 311
    • MC1066+pBS1539 (AmpR+URA3-Kl, TAP tag)
  • FB2306 = NB312
    • MC1066+pBS1479(AmpR+TRP1-Kl, TAP tag)
    • ref for seq of TRP1 from Kluyveromyces lactis here
    • NCBI link for seq of TRP1 from Kluyveromyces lactis here
from Methods 2001 article[1]
  • NB318
    • XL1-bl+pBS1479 (Lisa's prep of plasmid which does give PCR product for TAP-TRP, freshly transformed)

Yeast

  • FY631 = Parental for TAP tagging = NY411
    • MATa, his4-917d, lys2-173R2, leu2d1, ura3-52, trp1d63
  • FY2714 = NY412
    • MATa, HA-SPT3-TAP::TRP1, his4-917d, lys2-173R2, ura3D0 or -52, leu2D1 or D0, trp1D63
  • FY2031 = NY413
    • MATa, HA-SPT7-TAP::TRP1, his4-917d, lys2-173R2, ura3D0, leu2D1, trp1D63
  • FY2305 = NY414
    • MATa, SPT10-TAP::TRP1 trp1D63 his3D200 leu2D1 ura3-52 lys2-128d
    • not his4-912d
  • FY2306 = NY415
    • MATa, SPT21-TAP::TRP1 trp1D63 his3D200 leu2D1 ura3-52 lys2-128d
    • not his4-912d

Primers for C-terminal fusions

General format for
  • Upstream primer: 40nt then TCC ATG GAA AAG AGA AG
  • Downstream primer: 40nt then TAC GAC TCA CTA TAG GG
Relevant sequence files
  1. sequence of TAP tag only here
  2. sequence of pBS1479 here
from [2]
from [3]
Needed primers
needed to forward primer (5' to 3') reverse primer (5' to 3'
add TAP TRP to C-term of unknown 8 NO222
GGT ATT TGT CGA TTA CAA AAC ACA TCC TGT AGG CGC AAA TTC CAT GGA AAA GAG AAG
57 mer
Tm = 66.7
landing Tm (17bases only) = 45.5 		NO223

GTT AGG ATT CAG TAC TAA CAC ATT CTC TAT GAC ACA ACC TTA CGA CTC ACT ATA GGG
57 mer
Tm = 65.0
landing Tm (17bases only)= 46.1

check TAP NO224
TCC ATG GAA AAG AGA AGA TGG AAA AAG AAT TTC ATA GCC GTC TC
44 mer
Tm = 63.6
use with reverse primer from tagging PCR
NO225
TCA GGT TGA CTT CCC CGC GGA ATT CGC GTC TAC
33 mer
Tm = 67.9
use with fwd primer from tagging PCR
expect length of TAP seq + TRP K. l seq = 554 bps (from 2147 to 2701 in pBS1479)
add TAP TRP to C-term of RNT1 NO226
CTC ACA AAA GAA TAA GAA AAG AAA ATT CTC AGA TAC AAG CTC CAT GGA AAA GAG AAG
57 mer
Tm = 63.8
NO227
ATC AAT GCA AGT TCC ATC ATG GTT GTG TAA AAG GAA CGT TTA CGA CTC ACT ATA GGG
57 mer
Tm = 66.9
longer landing sequences TCC ATG GAA AAG AGA AGA TG = 20 mer fwd landing
Tm = 49.6 ºC 		TAC GAC TCA CTA TAG GGC GA = 20 mer rev landing
Tm = 54.3 ºC
Unknown 8 + longer landing sequences NO228
GT ATT TGT CGA TTA CAA AAC ACA TCC TGT AGG CGC AAA TTC CAT GGA AAA GAG AAG ATG
59 mer
Tm = 66.5 ºC 		NO229
TT AGG ATT CAG TAC TAA CAC ATT CTC TAT GAC ACA ACC TTA CGA CTC ACT ATA GGG CGA
59 mer
Tm = 66.6 ºC
RNT1 + longer landing sequences NO230
TCACAA AAGAATAAGA AAAGAAAATT CTCAGATACA AGC TCC ATG GAA AAG AGA AGA TG
59 mer
Tm = 64.4 ºC 		NO231
TCA ATG CAA GTT CCA TCA TGG TTG TGT AAA AGG AAC GTT TAC GAC TCA CTA TAG GGC GA
59 mer
Tm = 68.4 ºC
check TAP NO258 for SPT3-TAP control
TTT AAA GGT GGT AGA CTC AGT TCT AAA CCA ATT ATC ATG tcc atg gaa aag aga aga tg
59 mer
use with NO225 = reverse primer for checking TAP tag
expect length of TAP seq + TRP K. l seq = 554 bps (from 2147 to 2701 in pBS1479)
NO259for SPT7-TAP control
AAT AGT TCA TTT AGC TTG AGC CTT CCT CGC CTT AAT CAA tcc atg gaa aag aga aga tg
59 mer
use with NO225 = reverse primer for checking TAP tag
expect length of TAP seq + TRP K. l seq = 554 bps (from 2147 to 2701 in pBS1479)
Check TAP with NO224 SPT3_check_rev
NO268
ACC AGA AGG AAA CCC ATG CAC CTC CAT GAT GAA ATT ATA CAA AAA T 		SPT7_check_rev
NO269
AGC AAA TGT ATT TAA TTA AAG ATA AAA TAT TCA ACT ATT TAG CGC GCT CA

Genes to tag

Option 1: S. cerevisiae SAGA subunits
Subunit size,chromosome,null p-type
Ada subunits
Ada1 (aka HFI1, SUP110, SRM12, GAN1) 1.467 kb=489 aa, Chr. XVI, viable
Ada2 (aka SWI8) 1.305 kb=434aa, Chr. IV, viable
Ada3(aka NGG1, SWI7) 2.109 kb=702aa, Chr. IV, viable
Gcn5 (aka ADA4, SWI9) 1.32 kb=439aa, Chr. VII, viable
Ada5 (aka SPT20) 1.815 kb=604aa, Chr. XV, viable
Spt subunits
Spt3 1.014 kb=337aa, Chr. IV, viable
Spt7(aka GIT2) 3.999 kb=1332aa, Chr. II, viable
Spt8 1.809 kb=602aa, Chr. XII, viable
Spt20 (aka Ada5) 1.815 kb=604aa, Chr. XV, viable
TAF subunits
TAF5 (aka TAF90) 2.397 kb=798aa, Chr. II, inviable
TAF6 (aka TAF60) 1.551 kb=516aa, Chr. VII, inviable
TAF9 (aka TAF17) 0.474 kb=157aa, Chr. XIII, inviable
TAF10 (aka TAF23, TAF25) 0.621 kb=206aa, Chr. IV, inviable
TAF12(aka TAF61, TAF68) 1.620 kb=539aa, Chr. IV, inviable
Tra subunit
Tra1 11.235 kb=3744aa, Chr. VIII, inviable
Other subunits
Sgf73 1.974 kb=657aa, Chr. VII , viable
Sgf29 0.779 kb=259aa, Chr. III, viable
Sgf11 0.3 kb=99aa, Chr.XVI, viable
Ubp8 1.416 kb=471aa, Chr. XIII, viable
Sus1 gene with intron, Chr. II, viable
Option 2: Unknown ORFs from SGF73/sgf73 array
Unknown ORF SGF73 green signal sgf73 red signal log2 (green/red)
1 YHR033W 38938 and 69586 285 and 570 7.1 and 6.9
2 YOR302W 3374 and 6054 49 and 167 6.1 and 5.2
3 YJR097W 524 and 1052 13 and 28 5.3 and 5.2
4 YBL028C 1146 and 2706 32 and 323 5.2 and 3.1
5 YDR034W-B 17290 447 5.3
6 YGR067C 12025 320 5.2
7 YKL037W 8340 282 4.9
8 YER067W 6296 and 12450 82556 and 81036 -3.7 and -2.7
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