Oncoprotein 18 levels and phosphorylation mediate megakaryocyte polyploidization in human erythroleukemia cells

␣Chang, Christina L.; Hora, N.A.; Huberman, Nina; Hinderer, Robert; KuKuruga, Mark; Hanash, Samir M.

doi:10.1002/1615-9861(200111)1:11<1415::aid-prot1415>3.0.co;2-f

Cited by 10 publications

(1 citation statement)

References 35 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…Studies of the expression of stress shock proteins and their functional regulation are an important field in cell biology . Protein expression during heat shock of Jurkat cells has been well characterized. − We already found that patterns of extraction proteins from heat-shock were differ from those from nontreated Jurkat cells. , In this time, the relation of heat-shock stress to Jurkat cells and apoptosis induction was investigated using the connected type of microdevice (Figure B).…”

Section: Resultsmentioning

confidence: 99%

Self-Contained On-Chip Cell Culture and Pretreatment System

Tabuchi

Baba

2004

J. Proteome Res.

View full text Add to dashboard Cite

In this study, we describe a simple on-chip cell culture and pretreatment system that requires no external machines. Conventional cell culture utilizes culture dishes or microtiter plates, where pipetting and centrifugation are indispensable for washing cells and changing media. However, our microdevice requires no external centrifugation or pump. Utilizing this microdevice, we attained dramatically shorter total analytical time with a high-throughput screening system for proteomic analysis (1 min per 12 samples; one eightieth of the conventional time). Protein expression of Jurkat cells during stress-shock induced apoptosis was readily analyzed using this system. We found that a seaweed extraction effectively induced apoptosis of Jurkat cells.

show abstract

Section: Resultsmentioning

confidence: 99%

Self-Contained On-Chip Cell Culture and Pretreatment System

Tabuchi

Baba

2004

J. Proteome Res.

View full text Add to dashboard Cite

show abstract

A protein molecular weight map of ES2 clear cell ovarian carcinoma cells using a two-dimensional liquid separations/mass mapping technique

Wang¹,

Kachman²,

Schwartz³

et al. 2002

Electrophoresis

View full text Add to dashboard Cite

A molecular weight map of the protein content of ES2 human clear cell ovarian carcinoma cells has been produced using a two-dimensional (2-D) liquid separations/mass mapping technique. This method uses a 2-D liquid separation of proteins from whole cell lysates coupled on-line to an electrospray ionization-time of flight (ESI-TOF) mass spectrometer to map the accurate intact molecular weight (M(r)) of the protein content of the cells. The two separation dimensions involve the use of liquid isoelectric focusing as the first phase and nonporous silica reversed-phase high-performance liquid chromatography (HPLC) as the second phase of separation. The detection by ESI-TOF-MS provides an image of pI versus M(r) analogous to 2-D gel electrophoresis. Each protein is then identified based upon matrix-assisted laser desorption/ionization (MALDI)-TOF-MS peptide mapping and intact M(r) so that a standard map is produced against which other ovarian carcinoma cell lines can be compared. The accurate intact M(r) together with the pI fraction, and peptide map serve to tag the protein for future interlysate comparisons. An internal standard is also used to provide a means for quantitation for future interlysate studies. In the ES2 cell line under study it is shown that nearly 900 M(r) bands are detected over 17 pI fractions from pH 4 to 12 and a M(r) range up to 85 kDa and that around 290 of these bands can be identified using mass spectrometric based techniques. The protein M(r) is detected within an accuracy of 150 ppm and it is shown that many of the proteins in this human cancer sample are modified compared to the database. The protein M(r) map may serve as a highly reproducible standard Web-based method for comparing proteins from related human cell lines.

show abstract