Presentation is loading. Please wait.

Presentation is loading. Please wait.

Supplemental Materials of Two conserved oligosaccharyltransferase catalytic subunits required for N-glycosylation exist in Spartina alterniflora Luyi Jiang.

Published byEmma Green Modified over 7 years ago

Similar presentations

Presentation on theme: "Supplemental Materials of Two conserved oligosaccharyltransferase catalytic subunits required for N-glycosylation exist in Spartina alterniflora Luyi Jiang."— Presentation transcript:

1 Supplemental Materials of Two conserved oligosaccharyltransferase catalytic subunits required for N-glycosylation exist in Spartina alterniflora Luyi Jiang #,1, Xin Zhu #,1, Jinmei Chen 1, Deyue Yang 1, Changfang Zhou 1, Zhi Hong 1* 1 School of life sciences, Nanjing University, 2 Hankou Road, Nanjing, Jiangsu 210093, China

2 A B Figure S1. The schematic diagram of primer position for cloning SaSTT3A and SaSTT3B The primers for cloning SaSTT3A (A) and SaSTT3B (B)were marked. The arrows in the figure indicated the direction that the primers amplified. The primers on the first lines in both (A) and (B) were used for RACE to clone the sequences of 5 and 3 untranslated regions. The primers on the second lines were used for hi-TAIL to get the sequences in 5 end. The primers used for getting coding sequence and genomic DNA were listed in the third lines and fourth lines, respectively. Table S1 and S2 stated the above primers in detail.

3 Table S1 Primers for cDNA amplification Primer NamePrimer SequenceRemark cSaSTT3A-1F5’-GTTGCAGGCAGCTATGATAATG-3’ primers for CDS PCR cSaSTT3A-1R5’-CCAGAAATGATGCGAAGTGCTC-3’ cSaSTT3A-2F5’-TGGGCRGCAGCTGAAGCGTAC-3’ primers for CDS PCR cSaSTT3A-2R5’-ACCACCTCCTAGCGAACCATCC-3’ LAD15’-ACGATGGACTCCAGAG (G/C/A)N(G/C/A)NNNGGAA-3’ arbitrary degenerate primers for hi-TAIL PCR LAD25’-ACGATGGACTCCAGAG (G/C/T)N(G/C/T)NNNGGTT-3’ LAD35’-ACGATGGACTCCAGAG(G/C/A)(G/C/A)N(G/C/A)NNNCCAA-3’ LAD45’-ACGATGGACTCCAGAG(G/C/T)(G/A/T)N(G/C/T)NNNCGGT-3’ AC5’-ACGATGGACTCCAGAG-3’ SaSTT3A-SPR05’-GTACTAATGCTGCCAGAAGTGTTCCC-3’ gene specific primers for hi- TAIL PCR SaSTT3A-SPR15’-ACGATGGACTCCAGTCGACCAGTTACGATACACAAGAGCAC-3’ SaSTT3A-SPR25’-GCGTTGCATAGAAGAGTGATCCAGTG-3’ UPML5’-CTAATACGACTCACTATAGGGCAAGCAGTGGTATCAACGCGAGT-3’ adaptor primers for RACE UPMS5’-CTAATACGACTCACTATAGGGC-3’ ASP5’-AAGCAGTGGTATCAACGCAGAGTAC-3’ SaSTT3A-5GSPR15’-CCAGAAATGATGCGAAGTGCTC-3’ gene specific primers for RACE SaSTT3A-5GSPR25’-TAACCTCCCCAGGAGCAGACC-3’ SaSTT3A-3GSPF15’-AGTGGCAGAGAGTGCTTCTG-3’ SaSTT3A-3GSPF25’-AGGTTGCTTCCTGGTGGGACTATG-3’ cSaSTT3B-1F5’-GCATCGATGAATTCTCACSTTCTACYTCTTCGTG-3’ primers for CDS PCR cSaSTT3B-1R5’-GCTCTAGACTCGAGAAGCAGRGAGTAAAAYCGTC-3’ cSaSTT3B-2F5’-TGAAATACATGCTAAATGATGCCAG-3’ primers for CDS PCR cSaSTT3B-2R5’-ATAGCHGCATTSTGTTGGAATGG-3’ cSaSTT3B-3F15’-ATGGTGCGGTTAATTCTTGTTGCAGCAC-3’ primers for CDS PCR cSaSTT3B-3F25’-TACACTGCACTTGGGTGACATCTGAGGC-3’ cSaSTT3B-3R5’-THGGGGGTTTSACCTTGTATATGCGCAC-3’ SaSTT3B- SPR05’-AAAACCTGTAACAGGAAGAAGACTCCC-3’ gene specific primers for hi- TAIL PCR SaSTT3B- SPR15’-ACGATGGACTCCAGTCCAGAGTYCCAAGCACATACATGC-3’ SaSTT3B- SPR25’-TAGAAGTAGCCGAAGGCCGAGGC-3’ SaSTT3B-5GSPR15’-AAAACCTGTAACAGGAAGAAGACTCCC-3’ gene specific primers for RACE SaSTT3B-5GSPR25’-TAGAAGTAGCCGAAGGCCGAGGC-3’ SaSTT3B-3GSPF15’-TACACTGCACTTGGGTGACATCTGAAGC-3’ SaSTT3B-3GSPF25’CAACAGAGTATGGAAAACCTCCAGC-3’

4 Table S2 Primers for genomic DNA amplification Primer NamePrimer SequenceRemark gSaSTT3A-1F5’-TGGCGGGAAACTCCGCAAC-3’ primers for gDNA PCR gSaSTT3A-1R5’-CCAGAAATGATGCAAAGTGCTC-3’ gSaSTT3A-1S5’-CTTCCTGGGCTACTTACCTC-3’primer for sequencing gSaSTT3A-2F5’-TGCAGGCAGCTATGATAATGAAG-3’ primers for gDNA PCR gSaSTT3A-2R5’-TCAGACAAAGGCAAGAAGCATG-3’ gSaSTT3A-2S5’-GTCGTTACTCTTCACGAC-3’primer for sequencing gSaSTT3A-3F5’-ACATCCCCATCATCGCCAGTG-3’ primers for gDNA PCR gSaSTT3A-3R5’-TGTCATCACTAGGGTAGCCAA-3’ gSaSTT3A-3S15’-ACAATTGAAGGAGCCGAGTACGC-3’ primers for sequencing gSaSTT3A-3S25’-AGTGGCAGAGAGTGCTTCTG-3’ gSaSTT3A-4F5’-AGGTTGCTTCCTGGTGGGACTATG-3’ primers for gDNA PCR gSaSTT3A-4R5’-GGGGTACCCTATTGCCATGGGTTCTTTCG-3’ gSaSTT3B-1F5’-AGTCCAACTCCTCGCTAAGC-3’ primers for gDNA PCR gSaSTT3B-1R5’-AATCTGTTTCACCAGCATGCC-3’ gSaSTT3B-1S15’-GCATCGATGAATTCTCACSTTCTACYTCTTCGTG-3’ primers for sequencing gSaSTT3B-1S25’-GCTCTAGACTCGAGAAGCAGRGAGTAAAAYCGTC-3’ gSaSTT3B-2F5’-TGAAATACATGCTAAATGATGCCAG-3’ primers for gDNA PCR gSaSTT3B-2R5’-ACACTGCTCTTGAACTTGTG-3’ gSaSTT3B-2S15’-ACATAATTCACATCCAGTG-3’ primers for sequencing gSaSTT3B-2S25’-ATGGTGCGGTTAATTCTTGTTGCAGCAC-3’ gSaSTT3B-3F5’-TACACTGCACTTGGGTGACATCTGAGGC-3’ primers for gDNA PCR gSaSTT3B-3R5’-TCAGGACCTGTTCTTAGGGGGTTT-3’ gSaSTT3B-3S5’-THGGGGGTTTSACCTTGTATATGCGCAC-3’primer for sequencing gSaSTT3B-4F5’-CTGGACACTGTGATCTTTCCTG-3’ primers for gDNA PCR gSaSTT3B-4R5’-AGGAGTGTTCTGACGAAGCC-3’ gSaSTT3B-4S5’-GCTGGGCTGTCATTATTAGGAA-3’primer for sequencing

5 Table S3 Primers of construction for 35S:SaSTT3A/SaSTT3B, AtSTT3A:SaSTT3A/3B and RT-PCR Primer NamePrimer SequenceRemark SaSTT3A-Kpn Ⅰ -F 5’-GGGGTACCATGGCGGAGCCCGATGTGTCC-3’ primers for construction of 35S:SaSTT3A SaSTT3A-Sal Ⅰ -R 5’-GCGTCGACCTATTGCCATGGGTTCTTTCG-3’ SaSTT3B-EcoR Ⅰ -F 5’-CGAATTCATGGCGACCGCCGCGCTGGACTTCC-3’ primers for construction of 35S:SaSTT3B SaSTT3A-Pst Ⅰ -R 5’-AACTGCAGCACCTCAGGACCTGTTCTTAGG-3’ SaSTT3A-Afl Ⅱ -F 5’-TTACTTAAGAAATGGCGGAGCCCGATGTGTCC-3’ primers for construction of AtSTT3A:SaSTT3A SaSTT3A-Nhe Ⅰ -R 5’-CTAGCTAGCTATTGCCATGGGTTCTTTCG-3’ SaSTT3B-Afl Ⅱ -F 5’-TTACTTAAGATGGCGACCGCCGCGCTGGACTTCC-3’ primers for construction of AtSTT3A:SaSTT3B SaSTT3B-Nhe Ⅰ -R 5’- GGCTAGCACCTCAGGACCTGTTCTTAG-3’ cSaSTT3A-spe-F5’-AGTGTTGCCAGTACAAGCTC-3’ primers for RT-PCR of SaSTT3A cSaSTT3A-spe-R5’-TGTCATCACTAGGGTAGCCAA-3’ cSaSTT3B-spe-F5’-GTAAAAGCCCGCAGGTTGC-3’ primers for RT-PCR of SaSTT3B cSaSTT3B-spe-R5’-CATTGCACGCCCAACAGTAG-3’ cAtSTT3A-spe-F5’-ATTGCAAGTGTCAGTGAACATCAAC-3’ primers for RT-PCR of AtSTT3A cAtSTT3A-spe-R5’-CCTTGTCAGTCTTACCAGCAGAA-3’

Download ppt "Supplemental Materials of Two conserved oligosaccharyltransferase catalytic subunits required for N-glycosylation exist in Spartina alterniflora Luyi Jiang."

Similar presentations

RAPD Randomly Amplified Polymorphic DNA

RAPD Randomly Amplified Polymorphic DNA
BME 130 – Genomes Lecture 7 Genome Annotation I – Gene finding & function predictions.

BME 130 – Genomes Lecture 7 Genome Annotation I – Gene finding & function predictions.
PCR. PCR AMPLIFICATION PCR APPLICATIONS b MOLECULAR BIOLOGY b ENVIRONMENTAL SCIENCE b FORENSIC/MEDICAL SCIENCE b BIOTECHNOLOGY b GENETICS b GENE CLONING.

PCR. PCR AMPLIFICATION PCR APPLICATIONS b MOLECULAR BIOLOGY b ENVIRONMENTAL SCIENCE b FORENSIC/MEDICAL SCIENCE b BIOTECHNOLOGY b GENETICS b GENE CLONING.
Fig. S1 A622 1 MVVSEKSKILIIGGTGYIGKYLVETSAKSGHPTFALIRESTLKNPEKSKLIDTFKSYGVT 60 A622L 1..................................V.......V................. 60 A622.

Fig. S1 A622 1 MVVSEKSKILIIGGTGYIGKYLVETSAKSGHPTFALIRESTLKNPEKSKLIDTFKSYGVT 60 A622L V V A622.
Remember the limitations? –You must know the sequence of the primer sites to use PCR –How do you go about sequencing regions of a genome about which you.

Remember the limitations? –You must know the sequence of the primer sites to use PCR –How do you go about sequencing regions of a genome about which you.
Expression of the Genome The transcriptome. Decoding the Genetic Information  Information encoded in nucleotide sequences contained in discrete units.

Expression of the Genome The transcriptome. Decoding the Genetic Information  Information encoded in nucleotide sequences contained in discrete units.
Chapter 6 PCR and in vitro Mutagenesis A. Basic features of PCR 1. PCR is a cell-free method of DNA cloning standard PCR reaction is a selective DNA amplification.

Chapter 6 PCR and in vitro Mutagenesis A. Basic features of PCR 1. PCR is a cell-free method of DNA cloning standard PCR reaction is a selective DNA amplification.
Fig. S1 Mass spectra analysis of XXT4 reaction products demonstrating xylosyltransferase activity towards cellohexaose substrate. Predominant peaks represent.

Fig. S1 Mass spectra analysis of XXT4 reaction products demonstrating xylosyltransferase activity towards cellohexaose substrate. Predominant peaks represent.
Analysis of the atp9 5‘ trailer A B At5S-5 Atatp9.Endo.Mega.A atp9 At5S-Mega.R (-239) (-84/- 83) (+180) 5S rRNA 5’ 3’ atp9 mRNA atp9 pre-mRNA atp9 5’ leader.

Analysis of the atp9 5‘ trailer A B At5S-5 Atatp9.Endo.Mega.A atp9 At5S-Mega.R (-239) (-84/- 83) (+180) 5S rRNA 5’ 3’ atp9 mRNA atp9 pre-mRNA atp9 5’ leader.
The Polymerase Chain Reaction Some milestones In molecular biology recognised by the award of the Nobel prize.

The Polymerase Chain Reaction Some milestones In molecular biology recognised by the award of the Nobel prize.
Molecular Biology II Lecture 1 OrR. Restriction Endonuclease (sticky end)

Molecular Biology II Lecture 1 OrR. Restriction Endonuclease (sticky end)
東京大学 THE U NIVERSITY OF T OKYO Udayana University Amplifications of Terminal Ends of Newcastle Disease Virus Genome by Rapid Amplification of Complementary.

東京大学 THE U NIVERSITY OF T OKYO Udayana University Amplifications of Terminal Ends of Newcastle Disease Virus Genome by Rapid Amplification of Complementary.
0 0.1 0.2 0.3 0.4 0.5 0.6 WT#3#5#7#9#11#14#15#20#25#30 35S::JAZ13 Root length ratio * * * * * * * * * * Figure S2. Overexpression of native (untagged)

WT#3#5#7#9#11#14#15#20#25#30 35S::JAZ13 Root length ratio * * * * * * * * * * Figure S2. Overexpression of native (untagged)
Figure S1. RACE mapped transcription starts and polyA signals of Ogre CL5 and Ogre CL5del and putative splice site of Ogre CL5 and Ogre CL5del in Silene.

Figure S1. RACE mapped transcription starts and polyA signals of Ogre CL5 and Ogre CL5del and putative splice site of Ogre CL5 and Ogre CL5del in Silene.
Fig. S1: Fingerprinting of three BAC clones from different accessions of wild rice species with the AA genome constitution. The BAC DNAs were completely.

Fig. S1: Fingerprinting of three BAC clones from different accessions of wild rice species with the AA genome constitution. The BAC DNAs were completely.
MdSFBB3-alpha MSHVRESETPEDRVVEILSRLPPKSLMRFKCIHKSWFSLINNLSFVAKHLSNSVDNKLSSSTCILLNRSQAHIFPDQSWKQEVFWSMINFSIDSDENNLHYDVEDLN-IP 109 MdSFBB3-beta MSQVHESETPEDKVVEILCRLPPKSLMRFKCIRKSWCTLINRPSFVAKHLNNSVDNKLSSSTCILLNRSQAHIFPDQSWKQEVFWSTINLSIDSDEHNLHYDVEDLI-IP.

MdSFBB3-alpha MSHVRESETPEDRVVEILSRLPPKSLMRFKCIHKSWFSLINNLSFVAKHLSNSVDNKLSSSTCILLNRSQAHIFPDQSWKQEVFWSMINFSIDSDENNLHYDVEDLN-IP 109 MdSFBB3-beta MSQVHESETPEDKVVEILCRLPPKSLMRFKCIRKSWCTLINRPSFVAKHLNNSVDNKLSSSTCILLNRSQAHIFPDQSWKQEVFWSTINLSIDSDEHNLHYDVEDLI-IP.
Supplemental Fig. S1 A B AtMYBS1 3 57 128 180 314 aa AtMYBS2 7 58 112

Supplemental Fig. S1 A B AtMYBS aa AtMYBS
22 kDa a-coixin gene cluster

22 kDa a-coixin gene cluster
Quantitative Detection and Differentiation of Human Herpesvirus 6 Subtypes in Bone Marrow Transplant Patients by Using a Single Real-Time Polymerase Chain.

Quantitative Detection and Differentiation of Human Herpesvirus 6 Subtypes in Bone Marrow Transplant Patients by Using a Single Real-Time Polymerase Chain.
Schematic drawing of the human X chromosome and physical map the Xp interval carrying the ND gene. A 640-kb yeast artificial chromosome (YAC) clone was.

Schematic drawing of the human X chromosome and physical map the Xp interval carrying the ND gene. A 640-kb yeast artificial chromosome (YAC) clone was.

Similar presentations

Ads by Google