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PKC Isoform Expression in Modeled MicrogravityOur previous studies showed that modeled (MMG) and true (USA Space Shuttle Missions STS-54 and STS-56) microgravity (MG) inhibit human lymphocyte locomotion, Modeled MG also suppressed polyclonal and antigen-specific lymphocyte activation. Activation of PKC by phorbol myristate acetate (PMA) restored the microgravity-inhibited lymphocyte locomotion as well as activation by phytohaemagglutinin (PHA), whereas calcium ionophore (ionomycin) was unable to restore these functions. Based on these results we hypothesized that MG-induced changes in lymphocyte functions are caused by a fundamental defect in signal transduction mechanism. This defect may be localized either at the PKC level or upstream of PKC, most likely, at the cell membrane level. In this study we examined the expression of PKC isoforms alpha, epsilon and delta in PBMC cultured in rotating wall vessel bioreactor, developed at NASA JSC, which models microgravity by sustaining cells in continuous free fall. The assessment of the isoforms was performed by FACS analysis following cell permeabilization. A decrease in the expression of isoforms epsilon and delta, but not isoform a, was observed in PBMC cultured in microgravity conditions. These data suggest that MMG might selectively affect the expression of Ca2+ independent isoforms of PKC Molecular analysis confirm selective suppression of Ca2+ independent isoforms of PKC.
Document ID
20000105133
Acquisition Source
Johnson Space Center
Document Type
Preprint (Draft being sent to journal)
Authors
Risin, Diana
(Wyle Labs., Inc. Houston, TX United States)
Sundaresan, Alamelu
(Wyle Labs., Inc. Houston, TX United States)
Pellis, Neal R.
(NASA Johnson Space Center Houston, TX United States)
Dawson, David L.
Date Acquired
August 19, 2013
Publication Date
January 1, 1999
Subject Category
Space Processing
Funding Number(s)
CONTRACT_GRANT: NAG5-4072
CONTRACT_GRANT: NRA-OLMSA-02
Distribution Limits
Public
Copyright
Other

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