Literature DB >> 3294061

Morphological differentiation of embryonic rat sympathetic neurons in tissue culture. II. Serum promotes dendritic growth.

D A Bruckenstein1, D Higgins.   

Abstract

In the preceding paper, we reported that embryonic rat sympathetic neurons formed axons, but not dendrites, when they were maintained in the absence of serum and nonneuronal cells. To assess the effects of serum-derived factors on cellular morphology, cultures were initially maintained in serum-free medium while nonneuronal cells were eliminated. Subsequently some cultures were chronically exposed either to fetal calf serum (10%) or to a high-molecular-weight ammonium sulfate fraction of serum (P40 material, 500 micrograms/ml). Phase-contrast microscopy revealed that serum and P40 material did not alter neuronal survival, but did cause flattening of the somata and fasciculation of processes. When neurons exposed to serum or P40 material were injected with Lucifer Yellow, it was found that the majority (greater than or equal to 90%) had local, tapered processes that could be identified as dendrites by light microscopic criteria. These local processes also exhibited other dendritic characteristics in that (1) they reacted with monoclonal antibodies to nonphosphorylated forms of the M and H neurofilament subunits and to microtubule-associated protein 2; and (2) they had substantial amounts of RNA as determined by [3H]uridine autoradiography. Quantitative measurements of the effects of serum and P40 material on dendritic morphology revealed that (1) an 8-day exposure caused most neurons (greater than 80%) to form dendrites; (2) neurons typically had more than one dendrite (mean of 4.1 +/- 0.2 dendrites/cell after a 28-day exposure); and (3) the dendrites were relatively short with the maximum extent of the dendritic arbor being 110 +/- 13 micron after 4 weeks. Serum and P40 material did not routinely cause the formation of supernumerary axons, did not alter radial axonal outgrowth from ganglion explants, and did not significantly increase [3H]leucine incorporation. Thus, serum contains a factor (or factors) which selectively stimulates the extension of dendrites, but not axons. If such a factor were operative in situ, it could play an important role in determining the morphology of sympathetic neurons. In examining the mechanism of serum-induced dendritic growth, we found that even high concentrations (5 micrograms/ml) of nerve growth factor failed to promote dendritic growth in the absence of serum; thus, nerve growth factor by itself is not a sufficient condition for the extension of dendrites.(ABSTRACT TRUNCATED AT 400 WORDS)

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Year:  1988        PMID: 3294061     DOI: 10.1016/0012-1606(88)90296-5

Source DB:  PubMed          Journal:  Dev Biol        ISSN: 0012-1606            Impact factor:   3.582


  7 in total

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2.  MicroRNAs are Necessary for BMP-7-induced Dendritic Growth in Cultured Rat Sympathetic Neurons.

Authors:  Kristina Pravoverov; Katherine Whiting; Slesha Thapa; Trevor Bushong; Karen Trang; Pamela J Lein; Vidya Chandrasekaran
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3.  Interferon gamma induces retrograde dendritic retraction and inhibits synapse formation.

Authors:  In-Jung Kim; Hiroko Nagasawa Beck; Pamela J Lein; Dennis Higgins
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4.  Individual microtubules in the axon consist of domains that differ in both composition and stability.

Authors:  P W Baas; M M Black
Journal:  J Cell Biol       Date:  1990-08       Impact factor: 10.539

5.  A monoclonal anti-glycoconjugate antibody defines a stage and position-dependent gradient in the developing sympathoadrenal system.

Authors:  G A Schwarting; C M Story; G Deutsch
Journal:  Histochem J       Date:  1992-11

6.  The NC1 domain of type IV collagen promotes axonal growth in sympathetic neurons through interaction with the alpha 1 beta 1 integrin.

Authors:  P J Lein; D Higgins; D C Turner; L A Flier; V P Terranova
Journal:  J Cell Biol       Date:  1991-04       Impact factor: 10.539

7.  Unique responses of differentiating neuronal growth cones to inhibitory cues presented by oligodendrocytes.

Authors:  A Shibata; M V Wright; S David; L McKerracher; P E Braun; S B Kater
Journal:  J Cell Biol       Date:  1998-07-13       Impact factor: 10.539

  7 in total

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