MOLECULAR-CLONING AND FUNCTIONAL-CHARACTERIZATION OF CHICK LENS FIBER CONNEXIN-45.6

被引：84

作者：

JIANG, JX

WHITE, TW

GOODENOUGH, DA

PAUL, DL

机构：

[1] HARVARD UNIV,SCH MED,DEPT NEUROBIOL,BOSTON,MA 02115

[2] HARVARD UNIV,SCH MED,DEPT CELL BIOL,BOSTON,MA 02115

来源：

MOLECULAR BIOLOGY OF THE CELL | 1994年 / 5卷 / 03期

关键词：

D O I：

10.1091/mbc.5.3.363

中图分类号：

Q2 [细胞生物学];

学科分类号：

071009 ; 090102 ;

摘要：

The avian lens is an ideal system to study gap junctional intercellular communication in development and homeostasis. The lens is experimentally more accessible in the developing chick embryo than in other organisms, and chick lens cells differentiate well in primary cultures. However, only two members of the connexin gene family have been identified in the avian lens, whereas three are known in the mammalian system. We report here the molecular cloning and characterization of the third lens connexin, chick connexin45.6 (ChCx45.6), a protein with a predicted molecular mass of 45.6 kDa. ChCx45.6 was encoded by a single copy gene and was expressed specifically in the lens. There were two mRNA species of 6.4 kilobase (kb) and 9.4 kb in length. ChCx45.6 was a functional connexin protein, because expression in Xenopus oocyte pairs resulted in the development of high levels of conductance with a characteristic voltage sensitivity. Antisera were raised against ChCx45.6 and chick connexin56 (ChCx56), another avian lens-specific connexin, permitting the examination of the distribution of both proteins. Immunofluorescence localization showed that both ChCx45.6 and ChCx56 were abundant in lens fibers. Treatment of lens membranes with alkaline phosphatase resulted in electrophoretic mobility shifts, demonstrating that both ChCx45.6 and ChCx56 were phosphoproteins in vivo.

引用

页码：363 / 373

页数：11

共 61 条

[1] TRANSLATIONAL REGULATION OF DELTA-CRYSTALLIN SYNTHESIS DURING LENS DEVELOPMENT IN THE CHICKEN-EMBRYO
BEEBE, DC
PIATIGORSKY, J
[J]. DEVELOPMENTAL BIOLOGY, 1981, 84 (01) : 96 - 101
[2] BENNETT MVL, 1991, NEURON, V6, P305, DOI 10.1016/0896-6273(91)90241-Q
[3] Bennett MVL, 1978, NEUROSCI RES PROG B, V16, P373
[4] ANTISERA DIRECTED AGAINST CONNEXIN-43 PEPTIDES REACT WITH A 43-KD PROTEIN LOCALIZED TO GAP-JUNCTIONS IN MYOCARDIUM AND OTHER TISSUES
BEYER, EC
KISTLER, J
PAUL, DL
GOODENOUGH, DA
[J]. JOURNAL OF CELL BIOLOGY, 1989, 108 (02) : 595 - 605
[5] BEYER EC, 1990, J BIOL CHEM, V265, P14439
[6] CONNEXIN43 - A PROTEIN FROM RAT-HEART HOMOLOGOUS TO A GAP JUNCTION PROTEIN FROM LIVER
BEYER, EC
PAUL, DL
GOODENOUGH, DA
[J]. JOURNAL OF CELL BIOLOGY, 1987, 105 (06) : 2621 - 2629
[7] BEYER EC, 1990, J MEMBRANE BIOL, V116, P189
[8] CONNEXIN40, A COMPONENT OF GAP-JUNCTIONS IN VASCULAR ENDOTHELIUM, IS RESTRICTED IN ITS ABILITY TO INTERACT WITH OTHER CONNEXINS
BRUZZONE, R
HAEFLIGER, JA
GIMLICH, RL
PAUL, DL
[J]. MOLECULAR BIOLOGY OF THE CELL, 1993, 4 (01) : 7 - 20
[9] ISOLATION OF BIOLOGICALLY-ACTIVE RIBONUCLEIC-ACID FROM SOURCES ENRICHED IN RIBONUCLEASE
CHIRGWIN, JM
PRZYBYLA, AE
MACDONALD, RJ
RUTTER, WJ
[J]. BIOCHEMISTRY, 1979, 18 (24) : 5294 - 5299
[10] EXPRESSION OF FUNCTIONAL CELL-CELL CHANNELS FROM CLONED RAT-LIVER GAP JUNCTION COMPLEMENTARY-DNA
DAHL, G
MILLER, T
PAUL, D
VOELLMY, R
WERNER, R
[J]. SCIENCE, 1987, 236 (4806) : 1290 - 1293

← 1 2 3 4 5 6 7 →