EXPRESSION, PURIFICATION, AND CHARACTERIZATION OF THE DROSOPHILA KINESIN MOTOR DOMAIN PRODUCED IN ESCHERICHIA-COLI

被引:88
|
作者
GILBERT, SP [1 ]
JOHNSON, KA [1 ]
机构
[1] PENN STATE UNIV,DEPT MOLEC & CELL BIOL,106 ALTHOUSE LAB,UNIV PK,PA 16802
来源
BIOCHEMISTRY | 1993年 / 32卷 / 17期
关键词
D O I
10.1021/bi00068a028
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
The Drosophila kinesin heavy-chain gene was truncated to obtain the N-terminal 401 amino acid motor domain (designated K401) containing both the microtubule and ATP binding sites. The plasmid construct with the truncated kinesin gene was used to transform Escherichia coli. After induction, K401 was expressed as soluble kinesin protein at high levels and purified to homogeneity in milligram quantities. The purified protein was active and behaved as native kinesin with respect to its steady-state kinetic properties: K401 demonstrated a very low ATPase activity (k(cat) = 0.01 s-1) which was stimulated approximately 1000-fold by the addition of microtubules (k(cat) = 10 s-1; K0.5,MT = 0.9 muM tubulin; K(m,ATP) = 31 muM). Like native kinesin, K401 when purified contained ADP tightly bound at its active site, and the release of ADP from the active site occurred at a rate equal to the steady-state ATPase k(cat). Active-site measurements using [alpha-P-32]ATP demonstrated a stoichiometry of one ATPase site per K401 molecule. Like native kinesin, K401 can also hydrolyze MgGTP, and in the presence of microtubules, the rate of hydrolysis was increased dramatically from 0.03 to 16 s-1 (K0.5,MT = 2 muM tubulin; K(m,GTP) = 3.5 mM). These results establish that an active kinesin motor domain can be bacterially expressed and that this domain, the N-terminal 401 amino acids of the Drosophila kinesin heavy chain without light chains or additional eukaryotic factors, has full catalytic activity with microtubules. Furthermore, we found that truncation of the kinesin heavy chain to approximately 400 amino acids was necessary to purify the milligram amounts of active motor domain necessary for further mechanistic and structural studies to establish the basis for force production.
引用
收藏
页码:4677 / 4684
页数:8
相关论文
共 50 条
  • [1] DROSOPHILA KINESIN MINIMAL MOTOR DOMAIN EXPRESSED IN ESCHERICHIA-COLI - PURIFICATION AND KINETIC CHARACTERIZATION
    HUANG, TG
    HACKNEY, DD
    JOURNAL OF BIOLOGICAL CHEMISTRY, 1994, 269 (23) : 16493 - 16501
  • [2] EXPRESSION OF CATALYTICALLY ACTIVE HAMSTER DIHYDROOROTASE DOMAIN IN ESCHERICHIA-COLI - PURIFICATION AND CHARACTERIZATION
    WILLIAMS, NK
    YIN, PD
    SEYMOUR, KK
    RALSTON, GB
    CHRISTOPHERSON, RI
    PROTEIN ENGINEERING, 1993, 6 (03): : 333 - 340
  • [3] EXPRESSION, PURIFICATION, AND CHARACTERIZATION OF ESCHERICHIA-COLI DIHYDRODIPICOLINATE REDUCTASE
    REDDY, SG
    SACCHETTINI, JC
    BLANCHARD, JS
    BIOCHEMISTRY, 1995, 34 (11) : 3492 - 3501
  • [4] DROSOPHILA KINESIN MOTOR DOMAIN EXTENDING TO AMINO-ACID POSITION-392 IS DIMERIC WHEN EXPRESSED IN ESCHERICHIA-COLI
    HUANG, TG
    SUHAN, J
    HACKNEY, DD
    JOURNAL OF BIOLOGICAL CHEMISTRY, 1994, 269 (23) : 16502 - 16507
  • [5] PURIFICATION AND CHARACTERIZATION OF THE BACILLUS-SUBTILIS LEVANASE PRODUCED IN ESCHERICHIA-COLI
    WANKER, E
    HUBER, A
    SCHWAB, H
    APPLIED AND ENVIRONMENTAL MICROBIOLOGY, 1995, 61 (05) : 1953 - 1958
  • [6] PURIFICATION AND CHARACTERIZATION OF A SERRATIA-MARCESCENS NUCLEASE PRODUCED BY ESCHERICHIA-COLI
    BIEDERMANN, K
    JEPSEN, PK
    RIISE, E
    SVENDSEN, I
    CARLSBERG RESEARCH COMMUNICATIONS, 1989, 54 (01) : 17 - 27
  • [7] PURIFICATION AND CHARACTERIZATION OF HUMAN C5A PRODUCED IN ESCHERICHIA-COLI
    DAUMY, GO
    SCHULTE, GR
    MCCOLL, AS
    MERENDA, JM
    ANDREWS, GC
    GEOGHEGAN, KF
    DANLEY, DE
    SHOWELL, HJ
    ABSTRACTS OF PAPERS OF THE AMERICAN CHEMICAL SOCIETY, 1986, 192 : 7 - MBTD
  • [8] HIV NUCLEOCAPSID PROTEIN - EXPRESSION IN ESCHERICHIA-COLI, PURIFICATION, AND CHARACTERIZATION
    YOU, JC
    MCHENRY, CS
    JOURNAL OF BIOLOGICAL CHEMISTRY, 1993, 268 (22) : 16519 - 16527
  • [9] PURIFICATION OF RECOMBINANT ATRIOPEPTIGENS PRODUCED IN ESCHERICHIA-COLI
    SEETHARAM, R
    DEVINE, CS
    OLINS, PO
    BITTNER, ML
    WONG, EY
    BILD, GS
    GALLUPPI, GR
    AYKENT, S
    FOK, KF
    SMITH, CE
    ZURCHERNEELY, HA
    SIEGEL, NR
    HEEREN, RA
    BLEHM, DJ
    OLINS, GO
    GIERSE, JK
    ABSTRACTS OF PAPERS OF THE AMERICAN CHEMICAL SOCIETY, 1986, 192 : 15 - MBTD
  • [10] PURIFICATION AND CHARACTERIZATION OF THE HUMAN STROMELYSIN CATALYTIC DOMAIN EXPRESSED IN ESCHERICHIA-COLI
    YE, QZ
    JOHNSON, LL
    HUPE, DJ
    BARAGI, V
    BIOCHEMISTRY, 1992, 31 (45) : 11231 - 11235
12345