3 research outputs found
Antineoplastic effects of rosiglitazone and PPARγ transactivation in neuroblastoma cells
- Author
- A Chawla
- A Galli
- A Galli
- A Garaventa
- A Peri
- A Voigt
- B Desvergne
- B Farrow
- B Ottanelli
- C Grommes
- C J Thiele
- C Jiang
- C Jude-Aubry
- CF Chantrain
- CM Overall
- CP Reynolds
- D Shao
- DG Stupack
- DW Crabb
- E Ceni
- E Mueller
- F Cioppi
- G Debrock
- G Melino
- GD Demetri
- H Liu
- H Shimada
- H Yki-Järvinen
- HJ Burstein
- HP Koeffler
- I Cellai
- J Costa-Guda
- J Hisatake
- JO Nwako
- JR de Wet
- JR Gamble
- L Simi
- M Muratori
- M Serio
- MH Kulke
- MJ Reginato
- N Marx
- N Strakova
- P Ferruzzi
- P Luciani
- P Sarraf
- PJ Cox
- RA Gupta
- RA Ross
- S Baglioni
- S Benvenuti
- S Benvenuti
- SS Palakurthi
- SW Han
- T Servidei
- TG Kroll
- U Cavallaro
- U Valentiner
- V Carloni
- V Ciccarone
- Y Sugiura
- Publication venue
- Publication date
- Field of study
Get PDFNeuroblastoma (NB) is the most common extracranial solid tumour in infants. Unfortunately, most children present with advanced disease and have a poor prognosis. In the present study, we evaluated the role of the peroxisome proliferator-activated receptor γ (PPARγ) agonist rosiglitazone (RGZ) in two NB cell lines (SK-N-AS and SH-SY5Y), which express PPARγ. Rosiglitazone decreased cell proliferation and viability to a greater extent in SK-N-AS than in SH-SY5Y. Furthermore, 20 μM RGZ significantly inhibited cell adhesion, invasiveness and apoptosis in SK-N-AS, but not in SH-SY5Y. Because of the different response of SK-N-AS and SH-SY5Y cells to RGZ, the function of PPARγ as a transcriptional activator was assessed. Noticeably, transient transcription experiments with a PPARγ responsive element showed that RGZ induced a three-fold increase of the reporter activity in SK-N-AS, whereas no effect was observed in SH-SY5Y. The different PPARγ activity may be likely due to the markedly lower amount of phopshorylated (i.e. inactive) protein observed in SK-N-AS. To our knowledge, this is the first demonstration that the differential response of NB cells to RGZ may be related to differences in PPARγ transactivation. This finding indicates that PPARγ activity may be useful to select those patients, for whom PPARγ agonists may have a beneficial therapeutic effect
In vivo effects of rosiglitazone in a human neuroblastoma xenograft
- Author
- A Galli
- A Galli
- A Garaventa
- A Peri
- A Peri
- A Stojadinovic
- A Vecchi
- A Voigt
- AP Heaney
- AR Saltiel
- B De Bernardi
- B Desvergne
- B Heissig
- B Xin
- BM Spiegelman
- C Deledda
- C Grommes
- C Jiang
- C Jude-Aubry
- C Ricordati
- CF Chantrain
- CP Reynolds
- D Shao
- DG Stupack
- E Ceni
- E Mueller
- EJ Kim
- F Bogazzi
- F Cioppi
- G Bergers
- G Debrock
- G Melino
- G Petrangolini
- G Pratesi
- G Pratesi
- GD Demetri
- GP Bernini
- H Yki-Järvinen
- HG Burstein
- HP Koeffler
- I Cellai
- I Cellai
- J Hisatake
- J Roman
- JM Maris
- JO Nwankwo
- JR Weng
- JS Annicotte
- K Schultze
- KK Matthay
- M Balzi
- M Kato
- M Katoh
- M Ricote
- M Serio
- M Tortoreto
- M Vakkala
- MH Kulke
- MJ Reginato
- N Chattopadhyay
- N O’Donovan
- N Shimazaki
- P Faraoni
- P Luciani
- P Luciani
- P Tontonoz
- P Workman
- R Morosetti
- RA Nemenoff
- RM Cesario
- S Benvenuti
- S Gelmini
- S Hazra
- S Kersten
- SC Wong
- SM Hsu
- SS Palakurthi
- SW Han
- T Servidei
- T Yoshizumi
- TT Rohn
- U Valentiner
- VC Emmans
- VV Joshi
- W Kassouf
- Y Sugiura
- Y Tsubouchi
- Publication venue
- Nature Publishing Group
- Publication date
- Field of study
Get PDFRobust estimation of bacterial cell count from optical density
- Author
- Aarnio Tiu
- Aaron Leow Chung Yong
- Abbas Anser
- Abduraimova Aiganym
- Abraham Doris
- Acar Beliz Leyla
- Acosta Joaquin
- Adler Nina
- Adulyanukosol Natthawut
- Agena Ejouan
- Agena Ethan
- Aggarwal Priya
- Aguirre Adriana Lizeth Rubio
- Ahlgren Christopher
- Ahuja Janvi
- Aizik Dror
- Akbary Mina
- Akinfenwa Akinwumi
- Akingbesote Ngozi D.
- Akova Umut
- Aldo Ferdinan
- Alexopoulos Ioannis
- Allen Lucy
- Alonso Alejandro
- Altarawneh Dina
- Alvarado Andres Benjamin Sanchez
- Ambre Sanika
- Ameziane Annissa
- Amheine Khadija
- Amin Ihya Fakhrurizal
- Amir Sayeda Sakina
- Amstel Chiel van
- An Yongyan
- Anand Nithishwer Mouroug
- Ananthakrishnan Sathvik
- Anderson Karl
- Angel Sagi
- Annem Vidhya
- Anson Chung Tsun Ho
- Anwar Mariam
- Appel Alana
- Araya Lucas
- Armstrong Alexander
- Arora Neha
- Arora Vasu
- Arruda Beck
- Ashwin F Amal Jude
- Astapenka Artur
- Astles Ben
- Astorino Gabe
- Aubry Celine
- Avileli Rebecca
- Azad Mahnaz Sabeta
- Babar Rehmat
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- Zhou Yuxin
- Zhou Zhiyu
- Zhu Chushu
- Zhu Ke
- Zhu Xueqian
- Zi Lihan
- Zilinskaite Nemira
- Zimmermann Andreas
- Zimmermann Jennifer
- Zirong Zeng
- Ziwei Zhou
- Ziyi Zhao
- Zorrilla Francisco
- Zou Jiahua
- Zukauskaite Kristina
- Zulueta Patricia
- Zvirblyte Justina
- Publication venue
- Publication date
- 01/01/2020
- Field of study
Get PDFOptical density (OD) is widely used to estimate the density of cells in liquid culture, but cannot be compared between instruments without a standardized calibration protocol and is challenging to relate to actual cell count. We address this with an interlaboratory study comparing three simple, low-cost, and highly accessible OD calibration protocols across 244 laboratories, applied to eight strains of constitutive GFP-expressing E. coli. Based on our results, we recommend calibrating OD to estimated cell count using serial dilution of silica microspheres, which produces highly precise calibration (95.5% of residuals <1.2-fold), is easily assessed for quality control, also assesses instrument effective linear range, and can be combined with fluorescence calibration to obtain units of Molecules of Equivalent Fluorescein (MEFL) per cell, allowing direct comparison and data fusion with flow cytometry measurements: in our study, fluorescence per cell measurements showed only a 1.07-fold mean difference between plate reader and flow cytometry data
