Alpha 2.0
Login Register
» Articles » PMID: 14287179

OBSERVATIONS ON THE STRUCTURE OF RHODOSPIRILLUM MOLISCHIANUM

Overview
Journal J Cell Biol
Specialty Cell Biology
Date 1965 May 1
PMID 14287179
Citations 16
Authors
D D Hickman
A W Frenkel
Affiliations
Soon will be listed here.
Abstract

The lamellae of the bacterium Rhodospirillum molischianum originate as extensions of the cytoplasmic membrane into the cytoplasm of the cell. Initially, these extensions are narrow folds and occur independently of one another. The first lamellae to appear average about 80 A in width, representing one side of the infolded cytoplasmic membrane, or 160 A when the two sides of the fold are closely appressed. The 160-A lamellae increase in number and may associate to form larger lamellae, which represent varying degrees of association between adjacent folds. Later, the space within each fold increases; the two appressed regions of the cytoplasmic membrane in each fold separate to form distinct invaginations, and the lamellae observed at this stage are formed by an association of the sides of adjacent invaginations.

Citing Articles

Albert W. Frenkel (1919-2015): photosynthesis research pioneer, much-loved teacher, and scholar.

Govindjee , Frenkel S Photosynth Res. 2015; 124(3):243-7.

PMID: 25749907 DOI: 10.1007/s11120-015-0109-x.

Recollections.

Frenkel A Photosynth Res. 2013; 35(2):103-16.

PMID: 24318678 DOI: 10.1007/BF00014742.

Protein-induced membrane curvature investigated through molecular dynamics flexible fitting.

Hsin J, Gumbart J, Trabuco L, Villa E, Qian P, Hunter C Biophys J. 2009; 97(1):321-9.

PMID: 19580770 PMC: 2711417. DOI: 10.1016/j.bpj.2009.04.031.

Revealing linear aggregates of light harvesting antenna proteins in photosynthetic membranes.

He Y, Zeng X, Mukherjee S, Rajapaksha S, Kaplan S, Lu H Langmuir. 2009; 26(1):307-13.

PMID: 19572507 PMC: 2995330. DOI: 10.1021/la9012262.

Intrinsic curvature properties of photosynthetic proteins in chromatophores.

Chandler D, Hsin J, Harrison C, Gumbart J, Schulten K Biophys J. 2008; 95(6):2822-36.

PMID: 18515401 PMC: 2527265. DOI: 10.1529/biophysj.108.132852.

References
1.
Palade G . A study of fixation for electron microscopy. J Exp Med. 1952; 95(3):285-98. PMC: 2212069. DOI: 10.1084/jem.95.3.285. View
2.
Chapman G, Hillier J . Electron microscopy of ultra-thin sections of bacteria I. Cellular division in Bacillus cereus. J Bacteriol. 1953; 66(3):362-73. PMC: 357155. DOI: 10.1128/jb.66.3.362-373.1953. View
3.
Watson M . Staining of tissue sections for electron microscopy with heavy metals. J Biophys Biochem Cytol. 1958; 4(4):475-8. PMC: 2224499. DOI: 10.1083/jcb.4.4.475. View
4.
Kellenberger E, RYTER A, SECHAUD J . Electron microscope study of DNA-containing plasms. II. Vegetative and mature phage DNA as compared with normal bacterial nucleoids in different physiological states. J Biophys Biochem Cytol. 1958; 4(6):671-8. PMC: 2224514. DOI: 10.1083/jcb.4.6.671. View
5.
Watson M . Staining of tissue sections for electron microscopy with heavy metals. II. Application of solutions containing lead and barium. J Biophys Biochem Cytol. 1958; 4(6):727-30. PMC: 2224513. DOI: 10.1083/jcb.4.6.727. View