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Table A. Sequences used in making CsKASII RNAi constructs

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1 Table A. Sequences used in making CsKASII RNAi constructs
S1 File Table A. Sequences used in making CsKASII RNAi constructs 169 bp 5’ UTR sequence for RNAi-1 TTTTACGCATCGAAGGCTCTCTGCACGCCTCCTGAAAGAGAGAGAGAGAGAGAAGGAGAGAGAGATCATCACAGATCGATTCTCTCTTAAATCTCTCGTGAATCCCATTTCCCCTTCCGCTAGATTCTCTCTTCACTCATTTCTCGCTTTCTCTCCTTTTGTTCTCTCT 194 bp coding sequence for RNAi-2 AGGCGGAGATAGCCGCCAGGCTGCTGTCGCGCTTCAATCTGGTGGGCGGAGTCGGCGAAGGAGGCAGCTTACTAAATGCTCCTCTGCCTCTTCTCCTCCTCGATCCCCTTCCCCTCCTCCTACCATTCAAGCTCTTGTCTCTTCTTGTTTGGATTTTGGTCCTTGTACTCACTACTCCAACTCCAACTCCAACA

2 Table B. Primers used for gene detection
Primer name Primer sequence UcFATB1 UcFATB1-F1 5’- GAGAGAGTGCACGAGGGATA -3’ UcFATB1-R1 5’- CTGCAGGAATTCCCGATCTA -3’ CsKASII CsKASII-F1uni 5’- TTGCTACAAGGCAACAGTGG -3’ CsKASII-R1uni 5’ - AGACCTTCATCCCTCCCATT -3’ PP2A PP2A-qF1 5’ – TAACGTCGCCAAAATGATGC -3’ PP2A-qR1 5’ – GTTCTCCACAACCGATTGGT -3’

3 β-phas CsKASII 169 AtFAD2 intron Nos RNAi -1 RNAi-2 Figure A. CsKASII RNAi constructs. RNAi-1, β-phas, β-phaseolin gene promoter; CsKASII 169, 169 bp 5’UTR sequence of a CsKASII. B: RNAi-2, Napin, Napin promoter; CsKASII 194, 194 bp of coding sequence of a CsKASII. AtFAD2 intron, linker sequence used between two reversely oriented DNA fragments; Nos, nopaline synthase gene terminator. See details in the text.

4 A. UcFATB1 Napin  mCherry 35S RB NOS LB BamH I Probe B. Figure B. Southern analysis. A. T-DNA section of UcFATB1 overexpression construct. RB: Right Border; Napin: Napin promoter; UcFATB1: California bay 12:0-acyl-carrier protein thioesterase gene (NCBI GI:170555); 35S: cauliflower mosaic virus 35S promoter; mCherry: mCherry fluorescence gene; LB: Left Border. BamHI was used for genomic DNA digestion and the probe used in Southern was a fragment of UcFATB1 coding sequence. B. Southern blot analysis of three independent UcFATB1 transgenic lines (No. 4, 12 and 75) and a non-transgenic camelina plant (Wt). MW

5 Figure C. Relative expression of CsKASII gene in CsKASII RNAi transformed and wild type lines. RNA was extracted from T3 individual immature seeds days after pollination. Gene expression was measured by qRT-PCR SYBR Green method and normalized to PP2A expression.

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