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Barium action potentials in regenerating axons of the lamprey spinal cord

MacVicar BA; Llinas RR
Intracellular recordings were obtained from growing tips of regenerating giant axons in the lamprey spinal cord, the recording sites verified by Lucifer yellow injection. In the presence of extracellular Ba++ (3-6 mM), tetraethylammonium (10-15 mM), and 4-aminopyridine (4-6 mM), action potentials showed prolonged plateaus. The fast initial phase of the action potential, but not the plateau (Ba++-spike), was blocked by tetrodotoxin (10(-6) gm/ml). The Ba++ spike was associated with increased membrane conductance and could be terminated with hyperpolarizing current pulses. Normal axons did not generate similar Ba++ spikes. However, TTX-resistant, voltage-dependant conductance changes could be elicited in normal axons if much higher concentrations of Ba++ (18-30 mM) were used. Their rate of rise was slower than in regenerating axons (0.6 V/sec vs 3.2 V/sec; n = 5), and the response did not outlast the current pulse. The Ba++ responses in normal and regenerating axons were blocked by ions known to block voltage-gated Ca++ conductances (Co++, Ni++, or Cd++). Therefore, these spikes probably represent Ba++ entry through voltage-dependent Ca++ channels, suggesting the presence of a higher-than-average voltage-dependent Ca++ conductance in the growing axon. However, Ca++-dependent spikes could not be obtained under any conditions in either normal or regenerating axons. Simultaneous intracellular recordings from growth cones and axons indicated that the Ba++ spike was initiated, in most cases, at the growth cone. The Ba++ spikes were recorded in regenerating axons for as long as 50 days following cord transection and were not correlatable with the 'dying-back' phenomenon in cut axons, which usually is over before day 6. The concept of a higher-than-average voltage-dependent Ca++ conductance in growing tips of regenerating axons is in agreement with the hypothesis that Ca++ is important in regeneration and that regeneration may be related to the process of chemical synaptic transmission.
PMID: 2579243
ISSN: 0360-4012
CID: 9953

FURTHER-STUDIES ON THE EFFECT OF PRESYNAPTIC INJECTION OF SYNAPSIN-I AND CA/CALMODULIN-DEPENDENT KINASE-II (CAM KINASE-II) IN THE SQUID GIANT SYNAPSE [Meeting Abstract]

Llinas, R; Sugimori, M; Mcguinness, T; Gruner, J; Greengard, P
ISI:A1985AUC5500072
ISSN: 0006-3185
CID: 30711

Electronic transmission in the mammalian central nervous system

Chapter by: Llinas R
in: Gap junctions by Bennett MVL; Spray DC [Eds]
Cold Spring Harbor NY : Cold Spring Harbor Lab, 1985
pp. 337-353
ISBN: 0879691875
CID: 3274

Neuronal oscillators in mammalian brain

Chapter by: Llinas R
in: Comparative neurobiology : modes of communication in the nervous system by Cohen MJ; Strumwasser F; Bullock TH [Eds]
New York : Wiley, 1985
pp. 279-290
ISBN: 0471878537
CID: 3275

Functional significance of the basic cerebellar circuit in motor coordination

Chapter by: Llinas R
in: Cerebellar functions by Bloedel JR; Dichgans J; Precht W [Eds]
Berlin : Springer-Verlag, 1985
pp. 170-185
ISBN: 0387137289
CID: 3282

DIRECT DEMONSTRATION OF DENDRITIC INHIBITION IN CEREBELLAR PURKINJE CELLS IN-VITRO [Meeting Abstract]

SUGIMORI M; LLINAS R
BIOSIS:PREV198630085491
ISSN: 0190-5295
CID: 92435

SOME PROPERTIES OF AN ORGANOTYPIC CULTURE MODEL OF THE CEREBELLUM [Meeting Abstract]

KAPOOR R; JAEGER C B; LLINAS R
BIOSIS:PREV198630085490
ISSN: 0190-5295
CID: 92436

BURST FIRING PROPERTIES OF DEEP CEREBELLAR NUCLEI CELLS STUDIED IN THE ISOLATED GUINEA-PIG BRAINSTEM CEREBELLUM IN-VITRO [Meeting Abstract]

MUHLETHALER M; LLINAS R
BIOSIS:PREV198630085489
ISSN: 0190-5295
CID: 92437

CIRCUMVENTION OF DEHYDRATION-INDUCED MORPHOLOGICAL ARTIFACTS IN INTRACELLULARLY STAINED NEURONS BY A RAPID DMSO CLEARING PROCESS [Meeting Abstract]

GRACE A A; LLINAS R
BIOSIS:PREV198630077475
ISSN: 0190-5295
CID: 92438

EVIDENCE FOR DYNAMIC ELECTROTONIC COUPLING IN MAMMALIAN INFERIOR OLIVE IN-VIVO [Meeting Abstract]

SASAKI K; LLINAS R
BIOSIS:PREV198630070044
ISSN: 0190-5295
CID: 92439