2015
DOI: 10.1094/mpmi-05-14-0144-ta
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pFPL Vectors for High-Throughput Protein Localization in Fungi: Detecting Cytoplasmic Accumulation of Putative Effector Proteins

Abstract: As part of a large-scale project whose goal was to identify candidate effector proteins in Magnaporthe oryzae, we developed a suite of vectors that facilitate high-throughput protein localization experiments in fungi. These vectors utilize Gateway recombinational cloning to place a gene's promoter and coding sequences upstream and in frame with enhanced cyan fluorescent protein, green fluorescent protein (GFP), monomeric red fluorescence protein (mRFP), and yellow fluorescent protein or a nucleus-targeted mCHE… Show more

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Cited by 24 publications
(16 citation statements)
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“…The 1.3kb promoter of ChPKS38 was amplified with Phusion polymerase (ThermoFisher Scientific, Waltham, Massachusetts) using primer pair 1 and the 1.2kb 3' flanking region of ChPKS38 with primer pair 2. The mRFP and G418 resistance genes were amplified from the plasmid pFPL-Rg [59] with primer pairs 3 and 4, respectively. The four fragments were then joined using primer pair 5 by double-joint PCR [60].…”
Section: Methodsmentioning
confidence: 99%
“…The 1.3kb promoter of ChPKS38 was amplified with Phusion polymerase (ThermoFisher Scientific, Waltham, Massachusetts) using primer pair 1 and the 1.2kb 3' flanking region of ChPKS38 with primer pair 2. The mRFP and G418 resistance genes were amplified from the plasmid pFPL-Rg [59] with primer pairs 3 and 4, respectively. The four fragments were then joined using primer pair 5 by double-joint PCR [60].…”
Section: Methodsmentioning
confidence: 99%
“…Transformation cassettes to observe secretion in rice cells were constructed containing the entire protein coding sequence (including the predicted signal peptide) with its native promoter (1.1 kb) in a translational fusion with mRFP. The genomic sequence of MGG_09379 (SPD8, Bas162) was amplified using primers ISP2_F (aaaaagcaggcttaTTCCGATGATTCCCTCTGTC) and ISP2_R (agaaagctgggtaAGTGCTTTTAACCTGGTCCCA), cloned into the donor vector pDONR, and transferred into the destination vector pFPL‐Rh via Gateway cloning using the described methods (Gong et al ., ). The resulting plasmid (pBV921) was transformed into A. tumefaciens strain AGL1 cells and then incorporated into M. oryzae wild‐type strain O‐137 via Agrobacterium ‐mediated transformation with selection for hygromycin resistance (Khang et al ., ).…”
Section: Methodsmentioning
confidence: 97%
“…Plasmid pRF‐HUE‐YFP was constructed to express YFP in V. dahliae under the control of the glyceraldehyde 3‐phosphate dehydrogenase constitutive promoter of Aspergillus nidulans . The pair of primers YFP‐UserF (5′‐GGACTTAAUATGGTGAGCAAGGGCGAGGAG‐3′) and YFP‐UserR (5′‐GGGTTTAAUTTACTTGTACAGCTCGTCCATGCCG‐3′) was used to amplify a 720 bp DNA fragment containing the coding region of eYFP using the plasmid pFLG (Gong et al ., ) as template. Both primers included the sequences (underlined letters) needed to ligate the PCR product to plasmid pRF‐HUE digested with Pac I and Nt.Bbv CI USER enzymes (Frandsen et al ., ).…”
Section: Methodsmentioning
confidence: 99%