第22种氨基酸和无义密码子的重新诠释

遗传密码字典的破译,通用性作为遗传密码的基本特点之一被人们认可.近年来的研究发现了一些例外.除线粒体使用一组密码子其含义有别于核基因之外,原先被认为仅用作终止信号的无义密码子在某些情况下可重新诠释,编码特定的氨基酸.在揭示了硒代半胱氨酸由UGA编码后,最近的研究表明,在某些古细菌和真细菌中,无义密码子UAG可重新诠释,编码组成蛋白质的第22种天然氨基酸——吡咯赖氨酸.     

水稻线粒体tRNATrp突变体的克隆和氨酰化活力鉴定

为了研究tRNA^Trp的氨基酸接受茎中除两对半碱基以外的特异性元件,设计并完成了4种水稻线粒体tRNA^Trp向枯草杆菌tRNA^Trp的突变体 (MPB0, G1A和U5G/A68C;MPB1,C2G/G71C;MPB2,C4G/G69C;MPB3,C2G/G71C和C4G/G69C),体外转录并用枯草杆菌和人这两种不同种属来源的色氨酰 tRNA 合成酶(TrpRS)测定了这些 tRNA^Trp 分子的氨酰化活力(K_cat/K_M)．结果表明,这些突变体具有被枯草杆菌TrpRS氨酰化的能力,与野生型水稻线粒体tRNA^Trp相比,MPB0被枯草杆菌TrpRS氨酰化的活力提高了5倍,MPB1和MPB2被枯草杆菌TrpRS氨酰化的活力分别提高了40和53倍,MPB3则提高了140倍,为野生型枯草杆菌tRNA^Trp的34%,而人色氨酰 tRNA合成酶氨酰化这4个突变体的活力都很微弱．揭示了水稻线粒体tRNA^Trp氨基酸接受茎上的2个碱基对C2/G71和C4/G69的突变,对枯草杆菌TrpRS的识别起重要作用,由此推测,接受茎上的2个碱基对C2/G71和C4/G69也是线粒体tRNA^Trp重要的特异性元件．     

大肠杆菌等受体tRNALeu的T7 RNA聚合酶转录

用化学方法合成编码 2个大肠杆菌tRNA^Leu(tRNA^Leu₁和tRNA^Leu₂ )的基因和T7启动子 ,分别克隆到pUC1 9载体上 ,并在纯化的T7RNA聚合酶的体外转录系统中转录出不含修饰核苷酸的tRNA^Leu.在T7转录体系中 ,亚精胺对转录有负影响 .在最适转录条件下 ,可以得到有活力的RNA转录物的量是模板DNA的 2 5 0倍左右 .在大肠杆菌亮氨酰 tRNA合成酶的催化下 ,2种经体外转录产生的未修饰等受体tRNA^Leu(tRNA^Leu₁和tRNA^Leu₂ )的亮氨酸接受能力基本相同 ,但只有从体内纯化对应的tRNA^Leu的四分之一左右 ,表明修饰核苷酸在tRNA^Leu氨酰化过程中起着较为重要但非关键的作用 .     

大肠杆菌tRNALeu的基因克隆、高效表达和纯化

用化学法合成的tRNA^Leu 和tRNA^Leu ₂的基因分别连接到 pTrc99B质粒载体上 ,转化到大肠杆菌MT10 2中 .DNA测序筛选得到与已知tRNA^Leu₁ 和tRNA^Leu₂ 的基因顺序完全相同的克隆 .对带有tRNA^Leu₁ 和tRNA^Leu₂ 基因的 2个转化子 (MT -Leu1和MT- Leu2 )表达条件进行了优化 ,MT- Leu1和MT- Leu2总tRNA中的亮氨酸接受活力分别达到 810 pmol/A2 6 0 和 5 60 pmol/A2 6 0 :tRNA^Leu₁ 占MT -Leu1总tRNA的5 0 % ;tRNA^Leu₂ 占MT- Leu2总tRNA的 3 0 % .经DEAE Sepharose、BD -纤维素层析柱 ,可分别将MT- Leu1和MT -Leu2的总tRNA纯化到 160 0pmol/A2 6 0 .首次准确地测得了 2种等受体tRNALeu的氨酰化反应动力学常数 .     

基因编码的第22种氨基酸——吡咯赖氨酸

最近,来自俄亥俄州立大学两个研究小组的Hao等8位研究者鉴别出世界上第22种由遗传基因编码的天然氨基酸—吡咯赖氨酸(pyrrolysine)。 从1995年以来,Krzycki研究小组在对产甲烷甲胺(MMA,DMA,TMA)甲基转移酶     

牛肝TrnaIle的序列分析和二级结构

用随机降解法和Donis-Keller酶分析法,测定了牛肝tRNA^Ile序列.牛肝tRNA^Ile长77个碱基;G5·G69不配对为其显著特征.依据tRNA螺旋区和环区自由能大小及Holley模型,确定了tRNA^Ile的二级结构.     

E.coli tRNALeu的提纯

本文报道一种E.coli tRNA^Leu简便而稳定的纯化方法。粗tRNA经过BD-Cellulose柱层析和聚丙烯酰胺凝胶电泳两个步骤即可得到亮氨酸接受能力为1400pmol/A₂₆₀单位的tRNA^Leu。     

背瘤丽蚌F型线粒体基因组全序列分析

部分双壳贝类的线粒体遗传方式是特殊的双重单亲遗传方式:F型存在于雌性体细胞组织和性腺中,M型仅存在于雄性个体的性腺中。通过LA-PCR扩增、SHOT-GUN测序、软件拼接获得背瘤丽蚌(Lamprotula leai)F型线粒体基因组全序列。线粒体基因组全长为16530 bp,包括13个蛋白质编码基因,22个tRNA其中包括2个tRNA^Ser和2个tRNA^Leu,2个SrRNA及27个长度不等的非编码区,最长的两个非编码区分别为969 bp、228 bp。比较分析已登录到GenBank中的淡水蚌类F型线粒体结构特征,结果显示背瘤丽蚌F型A+T含量为60.28%,表现出A+T偏好性,淡水蚌类线粒体基因组长度的差异主要表现为非编码区长度的差异。此外,背瘤丽蚌mtDNA的COⅡ-12S rRNA区域基因排列存在差异,是ND3、tRNA^His、tRNA^Ala、tRNA^Ser1、tRNA^Ser2、tRNA^Glu、ND2、tRNA^Met 8个基因发生重排造成。F型线粒体序列构建的系统进化树中,淡水蚌类和海水双壳贝类分别聚为一支。研究结果为进一步研究淡水珍珠蚌的DUI线粒体遗传方式和种质资源保护奠定基础,为双壳贝类mtDNA基因重排提供依据。     

与耳聋相关的线粒体tRNA突变

线粒体tRNA基因突变是导致感音神经性耳聋的原因之一．有些tRNA突变可直接造成耳聋的发生,称之为原发突变．如tRNA^Leu(UUR) A3243G等突变与综合征型耳聋相关,而tRNA^Ser(UCN) T7511C等突变则与非综合征型耳聋相关．此外,继发突变如tRNA^Thr G15927A等突变则对原发突变起协同作用,影响耳聋的表型表达．这些突变可引起tRNA二级结构改变,从而影响线粒体蛋白质合成,降低细胞内ATP的产生,由此引起的线粒体功能障碍可导致耳聋的发生．主要讨论与耳聋相关的线粒体tRNA突变及其致聋机理．     

由tRNA引导的转录抗终止机制

由tRNA引导的转录抗终止机制普遍存在于革兰氏阳性细菌中,调控氨酰-tRNA合成酶基因和与氨基酸合成有关的酶基因的表达. 当某种氨基酸缺乏时,与其相关的tRNA增多. tRNA通过反密码子和3′接受末端与前导mRNA的特异序列和T框作用,促进前导mRNA中的终止子结构转变为抗终止子结构,使转录复合物能够通读,从而实现基因的表达.     

Specificity of Pyrrolysyl-tRNA Synthetase for Pyrrolysine and Pyrrolysine Analogs

Pyrrolysine, the 22nd amino acid, is encoded by amber (TAG = UAG) codons in certain methanogenic archaea and bacteria. PylS, the pyrrolysyl-tRNA synthetase, ligates pyrrolysine to tRNA^Pyl for amber decoding as pyrrolysine. PylS and tRNA^Pyl have potential utility in making tailored recombinant proteins. Here, we probed interactions necessary for recognition of substrates by archaeal PylS via synthesis of close pyrrolysine analogs and testing their reactivity in amino acid activation assays. Replacement of the methylpyrroline ring of pyrrolysine with cyclopentane indicated that solely hydrophobic interactions with the ring-binding pocket of PylS are sufficient for substrate recognition. However, a 100-fold increase in the specificity constant of PylS was observed with an analog, 2-amino-6-((R)-tetrahydrofuran-2-carboxamido)hexanoic acid (2Thf-lys), in which tetrahydrofuran replaced the pyrrolysine methylpyrroline ring. Other analogs in which the electronegative atom was moved to different positions suggested PylS preference for a hydrogen-bond-accepting group at the imine nitrogen position in pyrrolysine. 2Thf-lys was a preferred substrate over a commonly employed pyrrolysine analog, but the specificity constant for 2Thf-lys was 10-fold lower than for pyrrolysine itself, largely due to the change in K_m. The in vivo activity of the analogs in supporting UAG suppression in Escherichia coli bearing genes for PylS and tRNA^Pyl was similar to in vitro results, with l-pyrrolysine and 2Thf-lys supporting the highest amounts of UAG translation. Increasing concentrations of either PylS substrate resulted in a linear increase in UAG suppression, providing a facile method to assay bioactive pyrrolysine analogs. These results illustrate the relative importance of the H-bonding and hydrophobic interactions in the recognition of the methylpyrroline ring of pyrrolysine and provide a promising new series of easily synthesized pyrrolysine analogs that can serve as scaffolds for the introduction of novel functional groups into recombinant proteins.     

PylSn and the Homologous N-terminal Domain of Pyrrolysyl-tRNA Synthetase Bind the tRNA That Is Essential for the Genetic Encoding of Pyrrolysine

Pyrrolysine is represented by an amber codon in genes encoding proteins such as the methylamine methyltransferases present in some Archaea and Bacteria. Pyrrolysyl-tRNA synthetase (PylRS) attaches pyrrolysine to the amber-suppressing tRNA^Pyl. Archaeal PylRS, encoded by pylS, has a catalytic C-terminal domain but an N-terminal region of unknown function and structure. In Bacteria, homologs of the N- and C-terminal regions of archaeal PylRS are respectively encoded by pylSn and pylSc. We show here that wild type PylS from Methanosarcina barkeri and PylSn from Desulfitobacterium hafniense bind tRNA^Pyl in EMSA with apparent K_d values of 0.12 and 0.13 μm, respectively. Truncation of the N-terminal region of PylS eliminated detectable tRNA^Pyl binding as measured by EMSA, but not catalytic activity. A chimeric protein with PylSn fused to the N terminus of truncated PylS regained EMSA-detectable tRNA^Pyl binding. PylSn did not bind other D. hafniense tRNAs, nor did the competition by the Escherichia coli tRNA pool interfere with tRNA^Pyl binding. Further indicating the specificity of PylSn interaction with tRNA^Pyl, substitutions of conserved residues in tRNA^Pyl in the variable loop, D stem, and T stem and loop had significant impact in binding, whereas those having base changes in the acceptor stem or anticodon stem and loop still retained the ability to complex with PylSn. PylSn and the N terminus of PylS comprise the protein superfamily TIGR03129. The members of this family are not similar to any known RNA-binding protein, but our results suggest their common function involves specific binding of tRNA^Pyl.     

Recognition of Non-α-amino Substrates by Pyrrolysyl-tRNA Synthetase

Pyrrolysyl-tRNA synthetase (PylRS), an aminoacyl-tRNA synthetase (aaRS) recently found in some methanogenic archaea and bacteria, recognizes an unusually large lysine derivative, l-pyrrolysine, as the substrate, and attaches it to the cognate tRNA (tRNA^Pyl). The PylRS-tRNA^Pyl pair interacts with none of the endogenous aaRS-tRNA pairs in Escherichia coli, and thus can be used as a novel aaRS-tRNA pair for genetic code expansion. The crystal structures of the Methanosarcina mazei PylRS revealed that it has a unique, large pocket for amino acid binding, and the wild type M. mazei PylRS recognizes the natural lysine derivative as well as many lysine analogs, including N^?-(tert-butoxycarbonyl)-l-lysine (Boc-lysine), with diverse side chain sizes and structures. Moreover, the PylRS only loosely recognizes the α-amino group of the substrate, whereas most aaRSs, including the structurally and genetically related phenylalanyl-tRNA synthetase (PheRS), strictly recognize the main chain groups of the substrate. We report here that wild type PylRS can recognize substrates with a variety of main-chain α-groups: α-hydroxyacid, non-α-amino-carboxylic acid, N_α-methyl-amino acid, and d-amino acid, each with the same side chain as that of Boc-lysine. In contrast, PheRS recognizes none of these amino acid analogs. By expressing the wild type PylRS and its cognate tRNA^Pyl in E. coli in the presence of the α-hydroxyacid analog of Boc-lysine (Boc-LysOH), the amber codon (UAG) was recoded successfully as Boc-LysOH, and thus an ester bond was site-specifically incorporated into a protein molecule. This PylRS-tRNA^Pyl pair is expected to expand the backbone diversity of protein molecules produced by both in vivo and in vitro ribosomal translation.     

Distinct genetic code expansion strategies for selenocysteine and pyrrolysine are reflected in different aminoacyl-tRNA formation systems

Selenocysteine and pyrrolysine, known as the 21st and 22nd amino acids, are directly inserted into growing polypeptides during translation. Selenocysteine is synthesized via a tRNA-dependent pathway and decodes UGA (opal) codons. The incorporation of selenocysteine requires the concerted action of specific RNA and protein elements. In contrast, pyrrolysine is ligated directly to tRNA^Pyl and inserted into proteins in response to UAG (amber) codons without the need for complex re-coding machinery. Here we review the latest updates on the structure and mechanisms of molecules involved in Sec-tRNA^Sec and Pyl-tRNA^Pyl formation as well as the distribution of the Pyl-decoding trait.     

Crystallographic studies on multiple conformational states of active-site loops in pyrrolysyl-tRNA synthetase

Pyrrolysine, a lysine derivative with a bulky pyrroline ring, is the “22nd” genetically encoded amino acid. In the present study, the carboxy-terminal catalytic fragment of Methanosarcina mazei pyrrolysyl-tRNA synthetase (PylRS) was analyzed by X-ray crystallography and site-directed mutagenesis. The catalytic fragment ligated tRNA^Pyl with pyrrolysine nearly as efficiently as the full-length PylRS. We determined the crystal structures of the PylRS catalytic fragment in the substrate-free, ATP analogue (AMPPNP)-bound, and AMPPNP/pyrrolysine-bound forms, and compared them with the previously-reported PylRS structures. The ordering loop and the motif-2 loop undergo conformational changes from the “open” states to the “closed” states upon AMPPNP binding. On the other hand, the β7-β8 hairpin exhibits multiple conformational states, the open, intermediate (β7-open/β8-open and β7-closed/β8-open), and closed states, which are not induced upon substrate binding. The PylRS structures with a docked tRNA suggest that the active-site pocket can accommodate the CCA terminus of tRNA when the motif-2 loop is in the closed state and the β7-β8 hairpin is in the open or intermediate state. The entrance of the active-site pocket is nearly closed in the closed state of the β7-β8 hairpin, which may protect the pyrrolysyladenylate intermediate in the absence of tRNA^Pyl. Moreover, a structure-based mutational analysis revealed that hydrophobic residues in the amino acid-binding tunnel are important for accommodating the pyrrolysine side chain and that Asn346 is essential for anchoring the side-chain carbonyl and α-amino groups of pyrrolysine. In addition, a docking model of PylRS with tRNA was constructed based on the aspartyl-tRNA synthetase/tRNA structure, and was confirmed by a mutational analysis.     

In vivo identification of essential nucleotides in tRNALeu to its functions by using a constructed yeast tRNALeu knockout strain

The fidelity of protein biosynthesis requires the aminoacylation of tRNA with its cognate amino acid catalyzed by aminoacyl-tRNA synthetase with high levels of accuracy and efficiency. Crucial bases in tRNA^Leu to aminoacylation or editing functions of leucyl-tRNA synthetase have been extensively studied mainly by in vitro methods. In the present study, we constructed two Saccharomyces cerevisiae tRNA^Leu knockout strains carrying deletions of the genes for tRNA^Leu(GAG) and tRNA^Leu(UAG). Disrupting the single gene encoding tRNA^Leu(GAG) had no phenotypic consequence when compared to the wild-type strain. While disrupting the three genes for tRNA^Leu(UAG) had a lethal effect on the yeast strain, indicating that tRNA^Leu(UAG) decoding capacity could not be compensated by another tRNA^Leu isoacceptor. Using the triple tRNA knockout strain and a randomly mutated library of tRNA^Leu(UAG), a selection to identify critical tRNA^Leu elements was performed. In this way, mutations inducing in vivo decreases of tRNA levels or aminoacylation or editing ability by leucyl-tRNA synthetase were identified. Overall, the data showed that the triple tRNA knockout strain is a suitable tool for in vivo studies and identification of essential nucleotides of the tRNA.     

Rationally evolving tRNAPyl for efficient incorporation of noncanonical amino acids

Genetic encoding of noncanonical amino acids (ncAAs) into proteins is a powerful approach to study protein functions. Pyrrolysyl-tRNA synthetase (PylRS), a polyspecific aminoacyl-tRNA synthetase in wide use, has facilitated incorporation of a large number of different ncAAs into proteins to date. To make this process more efficient, we rationally evolved tRNA^Pyl to create tRNA^Pyl-opt with six nucleotide changes. This improved tRNA was tested as substrate for wild-type PylRS as well as three characterized PylRS variants (N^ϵ-acetyllysyl-tRNA synthetase [AcKRS], 3-iodo-phenylalanyl-tRNA synthetase [IFRS], a broad specific PylRS variant [PylRS-AA]) to incorporate ncAAs at UAG codons in super-folder green fluorescence protein (sfGFP). tRNA^Pyl-opt facilitated a 5-fold increase in AcK incorporation into two positions of sfGFP simultaneously. In addition, AcK incorporation into two target proteins (Escherichia coli malate dehydrogenase and human histone H3) caused homogenous acetylation at multiple lysine residues in high yield. Using tRNA^Pyl-opt with PylRS and various PylRS variants facilitated efficient incorporation of six other ncAAs into sfGFP. Kinetic analyses revealed that the mutations in tRNA^Pyl-opt had no significant effect on the catalytic efficiency and substrate binding of PylRS enzymes. Thus tRNA^Pyl-opt should be an excellent replacement of wild-type tRNA^Pyl for future ncAA incorporation by PylRS enzymes.     

Pyrrolysyl-tRNA synthetase: An ordinary enzyme but an outstanding genetic code expansion tool

The genetic incorporation of the 22nd proteinogenic amino acid, pyrrolysine (Pyl) at amber codon is achieved by the action of pyrrolysyl-tRNA synthetase (PylRS) together with its cognate tRNA^Pyl. Unlike most aminoacyl-tRNA synthetases, PylRS displays high substrate side chain promiscuity, low selectivity toward its substrate α-amine, and low selectivity toward the anticodon of tRNA^Pyl. These unique but ordinary features of PylRS as an aminoacyl-tRNA synthetase allow the Pyl incorporation machinery to be easily engineered for the genetic incorporation of more than 100 non-canonical amino acids (NCAAs) or α-hydroxy acids into proteins at amber codon and the reassignment of other codons such as ochre UAA, opal UGA, and four-base AGGA codons to code NCAAs.     

Probing unnatural amino acid integration into enhanced green fluorescent protein by genetic code expansion with a high-throughput screening platform

Background

Genetic code expansion has developed into an elegant tool to incorporate unnatural amino acids (uAA) at predefined sites in the protein backbone in response to an amber codon. However, recombinant production and yield of uAA comprising proteins are challenged due to the additional translation machinery required for uAA incorporation.

Results

We developed a microtiter plate-based high-throughput monitoring system (HTMS) to study and optimize uAA integration in the model protein enhanced green fluorescence protein (eGFP). Two uAA, propargyl-L-lysine (Plk) and (S)-2-amino-6-((2-azidoethoxy) carbonylamino) hexanoic acid (Alk), were incorporated at the same site into eGFP co-expressing the native PylRS/tRNA^Pyl _CUA pair originating from Methanosarcina barkeri in E. coli. The site-specific uAA functionalization was confirmed by LC-MS/MS analysis. uAA-eGFP production and biomass growth in parallelized E. coli cultivations was correlated to (i) uAA concentration and the (ii) time of uAA addition to the expression medium as well as to induction parameters including the (iii) time and (iv) amount of IPTG supplementation. The online measurements of the HTMS were consolidated by end point-detection using standard enzyme-linked immunosorbent procedures.

Conclusion

The developed HTMS is powerful tool for parallelized and rapid screening. In light of uAA integration, future applications may include parallelized screening of different PylRS/tRNA^Pyl _CUA pairs as well as further optimization of culture conditions.

     

Adding l-lysine derivatives to the genetic code of mammalian cells with engineered pyrrolysyl-tRNA synthetases

We report a method for site-specifically incorporating l-lysine derivatives into proteins in mammalian cells, based on the expression of the pyrrolysyl-tRNA synthetase (PylRS)-tRNA^Pyl pair from Methanosarcina mazei. Different types of external promoters were tested for the expression of tRNA^Pyl in Chinese hamster ovary cells. When tRNA^Pyl was expressed from a gene cluster under the control of the U6 promoter, the wild-type PylRS-tRNA^Pyl pair facilitated the most efficient incorporation of a pyrrolysine analog, N^ε-tert-butyloxycarbonyl-l-lysine (Boc-lysine), into proteins at the amber position. This PylRS-tRNA^Pyl system yielded the Boc-lysine-containing protein in an amount accounting for 1% of the total protein in human embryonic kidney (HEK) 293 cells. We also created a PylRS variant specific to N^ε-benzyloxycarbonyl-l-lysine, to incorporate this long, bulky, non-natural lysine derivative into proteins in HEK293. The recently reported variant specific to N^ε-acetyllysine was also expressed, resulting in the genetic encoding of this naturally-occurring lysine modification in mammalian cells.