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Dive into the research topics where Linn Hodneland Nilsson is active.

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Featured researches published by Linn Hodneland Nilsson.


PLOS ONE | 2014

Automated quantification and integrative analysis of 2D and 3D mitochondrial shape and network properties.

Julie Nikolaisen; Linn Hodneland Nilsson; Ina Katrine Nitschke Pettersen; Peter H. G. M. Willems; James B. Lorens; Werner J.H. Koopman; Karl Johan Tronstad

Mitochondrial morphology and function are coupled in healthy cells, during pathological conditions and (adaptation to) endogenous and exogenous stress. In this sense mitochondrial shape can range from small globular compartments to complex filamentous networks, even within the same cell. Understanding how mitochondrial morphological changes (i.e. “mitochondrial dynamics”) are linked to cellular (patho) physiology is currently the subject of intense study and requires detailed quantitative information. During the last decade, various computational approaches have been developed for automated 2-dimensional (2D) analysis of mitochondrial morphology and number in microscopy images. Although these strategies are well suited for analysis of adhering cells with a flat morphology they are not applicable for thicker cells, which require a three-dimensional (3D) image acquisition and analysis procedure. Here we developed and validated an automated image analysis algorithm allowing simultaneous 3D quantification of mitochondrial morphology and network properties in human endothelial cells (HUVECs). Cells expressing a mitochondria-targeted green fluorescence protein (mitoGFP) were visualized by 3D confocal microscopy and mitochondrial morphology was quantified using both the established 2D method and the new 3D strategy. We demonstrate that both analyses can be used to characterize and discriminate between various mitochondrial morphologies and network properties. However, the results from 2D and 3D analysis were not equivalent when filamentous mitochondria in normal HUVECs were compared with circular/spherical mitochondria in metabolically stressed HUVECs treated with rotenone (ROT). 2D quantification suggested that metabolic stress induced mitochondrial fragmentation and loss of biomass. In contrast, 3D analysis revealed that the mitochondrial network structure was dissolved without affecting the amount and size of the organelles. Thus, our results demonstrate that 3D imaging and quantification are crucial for proper understanding of mitochondrial shape and topology in non-flat cells. In summary, we here present an integrative method for unbiased 3D quantification of mitochondrial shape and network properties in mammalian cells.


Biochemical and Biophysical Research Communications | 2013

Induction of mitochondrial biogenesis and respiration is associated with mTOR regulation in hepatocytes of rats treated with the pan-PPAR activator tetradecylthioacetic acid (TTA).

Hanne R. Hagland; Linn Hodneland Nilsson; Lena Burri; Julie Nikolaisen; Rolf K. Berge; Karl Johan Tronstad

The hypolipidemic effect of peroxisome proliferator-activated receptor (PPAR) activators has been explained by increasing mitochondrial fatty acid oxidation, as observed in livers of rats treated with the pan-PPAR activator tetradecylthioacetic acid (TTA). PPAR-activation does, however, not fully explain the metabolic adaptations observed in hepatocytes after treatment with TTA. We therefore characterized the mitochondrial effects, and linked this to signalling by the metabolic sensor, the mammalian target of rapamycin (mTOR). In hepatocytes isolated from TTA-treated rats, the changes in cellular content and morphology were consistent with hypertrophy. This was associated with induction of multiple mitochondrial biomarkers, including mitochondrial DNA, citrate synthase and mRNAs of mitochondrial proteins. Transcription analysis further confirmed activation of PPARα-associated genes, in addition to genes related to mitochondrial biogenesis and function. Analysis of mitochondrial respiration revealed that the capacity of both electron transport and oxidative phosphorylation were increased. These effects coincided with activation of the stress related factor, ERK1/2, and mTOR. The protein level and phosphorylation of the downstream mTOR actors eIF4G and 4E-BP1 were induced. In summary, TTA increases mitochondrial respiration by inducing hypertrophy and mitochondrial biogenesis in rat hepatocytes, via adaptive regulation of PPARs as well as mTOR.


Scientific Reports | 2015

A new live-cell reporter strategy to simultaneously monitor mitochondrial biogenesis and morphology

Linn Hodneland Nilsson; Ina Katrine Nitschke Pettersen; Julie Nikolaisen; David R. Micklem; Hege Avsnes Dale; Gro Vatne Røsland; James B. Lorens; Karl Johan Tronstad

Changes in mitochondrial amount and shape are intimately linked to maintenance of cell homeostasis via adaptation of vital functions. Here, we developed a new live-cell reporter strategy to simultaneously monitor mitochondrial biogenesis and morphology. This was achieved by making a genetic reporter construct where a master regulator of mitochondrial biogenesis, nuclear respiratory factor 1 (NRF-1), controls expression of mitochondria targeted green fluorescent protein (mitoGFP). HeLa cells with the reporter construct demonstrated inducible expression of mitoGFP upon activation of AMP-dependent protein kinase (AMPK) with AICAR. We established stable reporter cells where the mitoGFP reporter activity corresponded with mitochondrial biogenesis both in magnitude and kinetics, as confirmed by biochemical markers and confocal microscopy. Quantitative 3D image analysis confirmed accordant increase in mitochondrial biomass, in addition to filament/network promoting and protecting effects on mitochondrial morphology, after treatment with AICAR. The level of mitoGFP reversed upon removal of AICAR, in parallel with decrease in mtDNA. In summary, we here present a new GFP-based genetic reporter strategy to study mitochondrial regulation and dynamics in living cells. This combinatorial reporter concept can readily be transferred to other cell models and contexts to address specific physiological mechanisms.


Current Pharmaceutical Design | 2014

Regulation and Quantification of Cellular Mitochondrial Morphology and Content

Karl Johan Tronstad; Marco Nooteboom; Linn Hodneland Nilsson; Julie Nikolaisen; Maciek Sokolewicz; Sander Grefte; Ina Katrine Nitschke Pettersen; Sissel E. Dyrstad; Fredrik Hoel; Peter H. G. M. Willems; Werner J.H. Koopman


Archive | 2017

Anti-axl antibodies

David Robert Micklem; Sergej Kiprijanov; Linn Hodneland Nilsson; Lavina Ahmed; Hallvard Haugen


Archive | 2017

ANTI-AXL ANTAGONISTIC ANTIBODIES

David Robert Micklem; Sergej Kiprijanov; James Bradley Lorens; Lavina Ahmed; Linn Hodneland Nilsson; Tone Sandal


Archive | 2017

SLFN11 AS BIOMARKER FOR AML

David Robert Micklem; Monica Hellesøy; Linn Hodneland Nilsson


Archive | 2017

ANTICORPS ANTAGONISTES ANTI-AXL

David Robert Micklem; Sergej Kiprijanov; James Bradley Lorens; Lavinia Ahmed; Linn Hodneland Nilsson; Tone Sandal


Scientific Reports | 2016

Corrigendum: A new live-cell reporter strategy to simultaneously monitor mitochondrial biogenesis and morphology

Linn Hodneland Nilsson; Ina Katrine Nitschke Pettersen; Julie Nikolaisen; David R. Micklem; Hege Avsnes Dale; Gro Vatne Røsland; James B. Lorens; Karl Johan Tronstad


Archive | 2016

Biomarkers for cancer

Monica Hellesøy; Linn Hodneland Nilsson; David Robert Micklem

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David Robert Micklem

University of Texas Southwestern Medical Center

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James Bradley Lorens

University of Texas Southwestern Medical Center

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