The role of the leucine zipper in the fos-jun interaction

Mutagenesis of the fos protein supports the hypothesis that a heptad repeat of leucine residues stabilizes the interaction between the fos and jun proteins. We show that the complex between fos and jun can bind to DNA more tightly than either protein alone and that basic residues adjacent to the leucine repeat of fos contribute to the DNA-binding potential of the complex.     

亮氨酸拉链结构蛋白在大肠杆菌重组子中的表达

酵母转录因子GCN4是通过亮氨酸拉链(bZIP)结构结合DNA的蛋白质之一，当GCN4二聚体与DNA结合时，亮氨酸拉链区的2个单体结合为平行的卷曲螺旋结构，而其基区由无规线团结构变为α螺旋．为探讨亮氨酸拉链蛋白与DNA的结合机理，设计了含有GCN4亮氨酸拉链蛋白基区结合DNA的必需氨基酸的折叠片段，并将其克隆到Escherichia coli BL21，讨论了此亮氨酸拉链蛋白的表达条件．在蛋白质的小量表达试验中，重组子Escherichia coli BL21于5mL含有50μg／mL氨节青霉素和34μg／mL氯霉素的LB液体培养基中培养至对数期，加入不同浓度的IPTG，继续培养以诱导蛋白质的表达，在不同的时间(如：诱导前，诱导2，4，6，8h)取样100μL到1．5mL离心管中、离心收集沉淀，将沉淀悬浮于样品缓冲液中，用10％SDS-PAGE检测；在10L含氨苄青霉素和氯霉素的LB液体培养基中进行了大量表达，根据小量表达的试验结果确定了IPTG的浓度和诱导时间．结果表明：含有这种拉链蛋白质的重组子Escherichia coli BL21在37℃下小量培养时，0．1-0．8mmol的IPTG均可在2-10h内诱导该蛋白质表达；而大量培养时，0．2mmol和0．4mmol的IPTG在37℃均不可能诱导表达，只在28℃时才表达；小量培养和大量培养的最佳诱导时间为4-6h，诱导剂IPTG的浓度为0．2mmol，大量表达的温度为28℃而不是37℃．     

Amino-terminal domains of c-myc and N-myc proteins mediate binding to the retinoblastoma gene product

The proteins encoded by the myc gene family are involved in the control of cell proliferation and differentiation, and aberrant expression of myc proteins has been implicated in the genesis of a variety of neoplasms. In the carboxyl terminus, myc proteins have two domains that encode a basic domain/helix-loop-helix and a leucine zipper motif, respectively. These motifs are involved both in DNA binding and in protein dimerization. In addition, myc protein family members share several regions of highly conserved amino acids in their amino termini that are essential for transformation. We report here that an N-terminal domain present in both the c-myc and N-myc proteins mediates binding to the retinoblastoma gene product, pRb. We show that the human papilloma virus E7 protein competes with c-myc for binding to pRb, indicating that these proteins share overlapping binding sites on pRb. Furthermore, a mutant Rb protein from a human tumour cell line that carried a 35-amino-acid deletion in its C terminus failed to bind to c-myc. Our results suggest that c-myc and pRb cooperate through direct binding to control cell proliferation.     

Contributions of a Position Amino Acid Residues to the Conformational Stability of GCN4 Leucine Zipper

Introduction Coiled coils[1] are widespread structures found in many natural proteins, such as structural proteins, transcrip- tion factors, receptor proteins, and enzymes[2,3]. Coils are the dominant structure in many fibrous proteins and the oligomeriza…     

大鼠肝再生相关基因MafF的分子进化研究

Maf家族是碱性亮氨酸拉链(the basic leucine zipper,bZip)转录因子的一个亚群,是v-maf癌蛋白类似物.它可以通过结合不同的底物来调节下游基因的表达.cDNA Microarray结果显示,小Maf家族成员MafF在大鼠部分肝切除后表达水平迅速升高.为了详细研究该基因的特性,我们采用生物信...     

ESCRT-III recognition by VPS4 ATPases

The ESCRT (endosomal sorting complex required for transport) pathway is required for terminal membrane fission events in several important biological processes, including endosomal intraluminal vesicle formation, HIV budding and cytokinesis. VPS4 ATPases perform a key function in this pathway by recognizing membrane-associated ESCRT-III assemblies and catalysing their disassembly, possibly in conjunction with membrane fission. Here we show that the microtubule interacting and transport (MIT) domains of human VPS4A and VPS4B bind conserved sequence motifs located at the carboxy termini of the CHMP1-3 class of ESCRT-III proteins. Structures of VPS4A MIT-CHMP1A and VPS4B MIT-CHMP2B complexes reveal that the C-terminal CHMP motif forms an amphipathic helix that binds in a groove between the last two helices of the tetratricopeptide-like repeat (TPR) of the VPS4 MIT domain, but in the opposite orientation to that of a canonical TPR interaction. Distinct pockets in the MIT domain bind three conserved leucine residues of the CHMP motif, and mutations that inhibit these interactions block VPS4 recruitment, impair endosomal protein sorting and relieve dominant-negative VPS4 inhibition of HIV budding. Thus, our studies reveal how the VPS4 ATPases recognize their CHMP substrates to facilitate the membrane fission events required for the release of viruses, endosomal vesicles and daughter cells.     

Portability of paddle motif function and pharmacology in voltage sensors

Voltage-sensing domains enable membrane proteins to sense and react to changes in membrane voltage. Although identifiable S1-S4 voltage-sensing domains are found in an array of conventional ion channels and in other membrane proteins that lack pore domains, the extent to which their voltage-sensing mechanisms are conserved is unknown. Here we show that the voltage-sensor paddle, a motif composed of S3b and S4 helices, can drive channel opening with membrane depolarization when transplanted from an archaebacterial voltage-activated potassium channel (KvAP) or voltage-sensing domain proteins (Hv1 and Ci-VSP) into eukaryotic voltage-activated potassium channels. Tarantula toxins that partition into membranes can interact with these paddle motifs at the protein-lipid interface and similarly perturb voltage-sensor activation in both ion channels and proteins with a voltage-sensing domain. Our results show that paddle motifs are modular, that their functions are conserved in voltage sensors, and that they move in the relatively unconstrained environment of the lipid membrane. The widespread targeting of voltage-sensor paddles by toxins demonstrates that this modular structural motif is an important pharmacological target.     

A protein binding to the J kappa recombination sequence of immunoglobulin genes contains a sequence related to the integrase motif

Site-specific recombination requires conserved DNA sequences specific to each system, and system-specific proteins that recognize specific DNA sequences. The site-specific recombinases seem to fall into at least two families, based on their protein structure and chemistry of strand breakage. One of these is the resolvase-invertase family, members of which seem to form a serine-phosphate linkage with DNA. Members of the other family, called the integrase family, contain a conserved tyrosine residue that forms a covalent linkage with the 3'-phosphate of DNA at the site of recombination. Structural comparison of integrases shows that these proteins share a highly conserved 40-residue motif. V-(D)-J recombination of the immunoglobulin gene requires conserved recombination signal sequences (RS) of a heptamer CACTGTG and a T-rich nonamer GGTTTTTGT, which are separated by a spacer sequence of either 12 or 23 bases We have recently purified, almost to homogeneity, a protein that specifically binds to the immunoglobulin J kappa RS containing the 23-base-pair spacer sequence. By synthesizing probes on the basis of partial amino-acid sequences of the purified protein, we have now isolated and characterized the complementary DNA of this protein. The amino-acid sequence deduced from the cDNA sequence reveals that the J kappa RS-binding protein has a sequence similar to the 40-residue motif of integrases of phages, bacteria and yeast, indicating that this protein could be involved in V-(D)-J recombination as a recombinase.     

高浓度c—Myc羧基端的体外自身二聚体化活性

将编码人c-myc羧基端bHLH／LZ结构域的92个氨基酸的cDNA片段（c-myc-c92）对框插入pGEX－2T原核表达载体中,使之与谷胱甘肽转移酶（GST）编码基因融合,并将重质粒导入大肠杆菌BL21（DE3）中,由IPTG诱导融合基因高效表达,并用Glutathione Sepharose4B亲和柱纯化融合蛋白GST－c-Myc-c92,凝胶阻滞（EMSA）分析显示该纯化蛋白能与CACGTG序列特异结合,并且只有高浓度的GST－c-Myc-c92才能与探针结合,结果表明在体上情况下高浓度c-Myc羟基端能自身二聚体化,此发现丰富了Myc-Max-Mad的调控网络,并为进一步研究c-myc的功能和调控提供了一定的线索。