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Dive into the research topics where Bo Johansen is active.

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Featured researches published by Bo Johansen.


Cell | 2000

Arabidopsis MAP Kinase 4 Negatively Regulates Systemic Acquired Resistance

Morten Petersen; Peter Brodersen; Henrik Næsted; Erik Andreasson; Ursula Lindhart; Bo Johansen; Henrik Bjørn Nielsen; Michelle Lacy; Mark J. Austin; Jane E. Parker; Sashi B. Sharma; Daniel F. Klessig; Robert A. Martienssen; Ole Mattsson; Anders Boeck Jensen; John Mundy

Transposon inactivation of Arabidopsis MAP kinase 4 produced the mpk4 mutant exhibiting constitutive systemic acquired resistance (SAR) including elevated salicylic acid (SA) levels, increased resistance to virulent pathogens, and constitutive pathogenesis-related gene expression shown by Northern and microarray hybridizations. MPK4 kinase activity is required to repress SAR, as an inactive MPK4 form failed to complement mpk4. Analysis of mpk4 expressing the SA hydroxylase NahG and of mpk4/npr1 double mutants indicated that SAR expression in mpk4 is dependent upon elevated SA levels but is independent of NPR1. PDF1.2 and THI2.1 gene induction by jasmonate was blocked in mpk4 expressing NahG, suggesting that MPK4 is required for jasmonic acid-responsive gene expression.


Plant Journal | 2008

Mixed‐linkage (1→3),(1→4)‐β‐d‐glucan is not unique to the Poales and is an abundant component of Equisetum arvense cell walls

Iben Sørensen; Filomena Pettolino; Sarah M. Wilson; Monika S. Doblin; Bo Johansen; Antony Bacic; William G. T. Willats

Mixed-linkage (1-->3),(1-->4)-beta-D-glucan (MLG) is widely considered to be a defining feature of the cell walls of plants in the Poales order. However, we conducted an extensive survey of cell-wall composition in diverse land plants and discovered that MLG is also abundant in the walls of the horsetail Equisetum arvense. MALDI-TOF MS and monosaccharide linkage analysis revealed that MLG in E. arvense is an unbranched homopolymer that consists of short blocks of contiguous 1,4-beta-linked glucose residues joined by 1,3-beta linkages. However, in contrast to Poaceae species, MLG in E. arvense consists mostly of cellotetraose rather than cellotetriose, and lacks long 1,4-beta-linked glucan blocks. Monosaccharide linkage analyses and immunochemical profiling indicated that, in E. arvense, MLG is a component of cell walls that have a novel architecture that differs significantly from that of the generally recognized type I and II cell walls. Unlike in type II walls, MLG in E. arvense does not appear to be co-extensive with glucuroarabinoxylans but occurs in walls that are rich in pectin. Immunofluorescence and immunogold localization showed that MLG occurs in both young and old regions of E. arvense stems, and is present in most cell types apart from cells in the vascular tissues. These findings have important implications for our understanding of cell-wall evolution, and also demonstrate that plant cell walls can be constructed in a way not previously envisaged.


Molecular Phylogenetics and Evolution | 2002

MADS-box gene evolution-structure and transcription patterns.

Bo Johansen; Louise B. Pedersen; Martin Skipper; Signe Frederiksen

This study presents a phylogenetic analysis of 198 MADS-box genes based on 420 parsimony-informative characters. The analysis includes only MIKC genes; therefore several genes from gymnosperms and pteridophytes are excluded. The strict consensus tree identifies all major monophyletic groups known from earlier analyses, and all major monophyletic groups are further supported by a common gene structure in exons 1-6 and by conserved C-terminal motifs. Transcription patterns are mapped on the tree to obtain an overview of MIKC gene transcription. Genes that are transcribed only in vegetative organs are located in the basal part of the tree, whereas genes involved in flower development have evolved later. As the universality of the ABC model has recently been questioned, special account is paid to the expression of A-, B-, and C-class genes. Mapping of transcription patterns on the phylogeny shows all three classes of MADS-box genes to be transcribed in the stamens and carpels. Thus the analysis does not support the ABC model as formulated at present.


Fungal Biology | 2002

In situ PCR for detection and identification of fungal species

Lene Bindslev; Richard P. Oliver; Bo Johansen

PCR and DNA sequence analysis have become standard tools for identification, detection and phylogenetic analysis of fungi. A large number of species are incapable of growth in the laboratory, making the preparation of pure DNA problematical. The amplification of DNA samples from impure material is subject to misinterpretation if more than one species is present. To overcome this problem, we designed an in situ PCR technique that links PCR amplification to the light microscopic image. The amplified tissue is stained, thus confirming which morphotype has been amplified. The PCR product can then be sequenced. We tested the technique on fixed Blumeria graminis spores and mycelia using primers derived from the sequence of the gene encoding the catalytic subunit of protein kinase A (bka1). This is the first report of in situ PCR on phytopathogenic fungal material. This technique allows positive confirmation of the origin of genes cloned from obligate pathogenic fungi and could be adapted for use on any samples containing mixed fungal species.


European Journal of Immunology | 2014

Midline 1 directs lytic granule exocytosis and cytotoxicity of mouse killer T cells

Lasse Boding; Ann Kathrine Hansen; Germana Meroni; Bo Johansen; Thomas Hartig Braunstein; Charlotte M. Bonefeld; Martin Kongsbak; Benjamin Anderschou Holbech Jensen; Anders Woetmann; Allan Randrup Thomsen; Niels Ødum; Marina Rode von Essen; Carsten Geisler

Midline 1 (MID1) is a microtubule‐associated ubiquitin ligase that regulates protein phosphatase 2A activity. Loss‐of‐function mutations in MID1 lead to the X‐linked Opitz G/BBB syndrome characterized by defective midline development during embryogenesis. Here, we show that MID1 is strongly upregulated in murine cytotoxic lymphocytes (CTLs), and that it controls TCR signaling, centrosome trafficking, and exocytosis of lytic granules. In accordance, we find that the killing capacity of MID1−/− CTLs is impaired. Transfection of MID1 into MID1−/− CTLs completely rescued lytic granule exocytosis, and vice versa, knockdown of MID1 inhibited exocytosis of lytic granules in WT CTLs, cementing a central role for MID1 in the regulation of granule exocytosis. Thus, MID1 orchestrates multiple events in CTL responses, adding a novel level of regulation to CTL activation and cytotoxicity.


Plant Journal | 2007

Disruption of ATCSLD5 results in reduced growth, reduced xylan and homogalacturonan synthase activity and altered xylan occurrence in Arabidopsis

Adriana J. Bernal; J. Jensen; Jesper Harholt; Susanne Sørensen; Isabel Moller; Claudia Blaukopf; Bo Johansen; Robert De Lotto; Markus Pauly; Henrik Vibe Scheller; William G. T. Willats


Gene | 2006

Cloning and transcription analysis of an AGAMOUS- and SEEDSTICK ortholog in the orchid Dendrobium thyrsiflorum (Reichb. f.).

Martin Skipper; Louise Kruse Johansen; Kim Blanksø Pedersen; Signe Frederiksen; Bo Johansen


Botanical Journal of the Linnean Society | 1990

Incompatibility in Dendrobium (Orchidaceae).

Bo Johansen


Annals of Botany | 1997

In situPCR on Plant Material with Sub-cellular Resolution

Bo Johansen


Plant Science | 2005

Identification and quantification of expression levels of three FRUITFULL-like MADS-box genes from the orchid Dendrobium thyrsiflorum (Reichb. f.)

Martin Skipper; Kim Blanksø Pedersen; Louise B. Johansen; Signe Frederiksen; Vivian F. Irish; Bo Johansen

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Martin Skipper

University of Copenhagen

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Antony Bacic

University of Melbourne

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