含羟基和咪唑基团新手性肽核酸的设计与合成

以含丝氨酸和组氨酸残基的手性肽核酸单体替换经典肽核酸单体, 采用固相合成方法设计合成了五个新序列含羟基和咪唑基团的10聚体手性肽核酸, 经ESI-MS或MALDI-TOF-MS证实目标物结构正确.     

手性膦肽核酸单体的合成

肽核酸是一种潜在的反义和反基因药物。膦肽结构的引入克服了肽核酸低水溶性和低细胞膜通透性等缺点,有利于肽核酸的应用。本研究报道手性磷肽核酸单体的合成。还原氨化方法被用于实现N-Boc,N-Fmoc保护的丙氨醛与甘氨膦酸二酯的偶联,BBC-Cl,FEP等缩合剂被用于实现碱基侧链和母链的高效缩合。     

肽核酸的合成、修饰和应用

肽核酸是寡核苷酸模拟物, 它的糖-磷酸骨架被N-(2-氨基乙基)甘氨酸骨架所代替. 为了优化肽核酸的性质, 各种结构的肽核酸(PNA)单体被合成出来. 综述了肽核酸的合成、结构修饰及应用.     

手性酰胺聚硅氧固定相的制备与气相色谱性能

以Ｌ－苯丙氨酸，Ｌ－缬氨酸为手性源，合成了二种含末端烯基，具有刚性苯基链节的新型手性酰胺单体；并通过硅氢加成方法将其接枝到含氢硅油上，制备了两种新型手性酰胺聚硅氧烷固定相。这一新方法具有简单易行，各步产率较高的优点，所制备了手性固定相具有较好的毛细管柱色谱性能。手性拆分能力和耐温性。     

基于原子转移自由基聚合和“Click”化学方法制备手性色谱固定相

应用原子转移自由基聚合(ATRP)法和"Click"化学方法,以含叠氮基的烯类化合物为单体,在硅胶表面引发聚合,制备了"梳状"手性固定相.该固定相的合成采用"接出"方法接枝聚合物链,使接枝层更为均匀,并且避免了传统合成方法(如物理吸附等)稳定性差的缺点.所得到的"梳状"手性固定相实现了对一些手性药物的分离;并考察了该固定相中聚合物链的密度和长度对其手性分离能力的影响.     

新型β-环糊精衍生物/硅基杂化手性固定相制备及评价

以脲氨基-β-环糊精硅基衍生物为手性单体,1,2-二(三乙氧基硅烷)乙烷(BTEE)为硅源,十六烷基三甲基溴化铵(CTAB)为模板,采用水热合成法制备脲氨基β-环糊精衍生物/硅基手性杂化材料(β-CD/PMOs)。以其为手性固定相制备一种新型毛细管电色谱开管柱,通过IR和SEM对固定相的结构和形貌进行表征。结果表明,固定相成功键合在毛细管内,并保留了固定相原有的球形结构。以硫脲为标记物,测得平均柱效在11698.4 plates/m以上,日内、日间及柱间柱效的相对标准偏差(RSD)(n=7)均≤1.31%,且成功拆分D,L-组氨酸,达到基线分离。可见,该开管柱具有良好的重现性、稳定性和手性拆分能力。     

手性酰胺聚硅氧烷固定相的制备与气相色谱性能

以L-苯丙氨酸,L-缬氨酸为手性源,合成了二种含末端烯基,具有刚性苯基链节的新型手性酰胺单体;并通过硅氢加成方法将其接枝到含氢硅油上,制备了两种新型手性酰胺聚硅氧烷固定相.这一新方法具有简单易行,各步产率较高的优点,所制备的手性固定相具有较好的毛细管柱色谱性能.手性拆分能力和耐温性.     

基于L-异亮氨酸衍生物的液晶单体及其聚合物的合成与结构表征

通过对L-异亮氨酸化合物进行扩展性研究及分子设计,本论文合成了四种含(2S,3S)-3-甲基-2-氯戊酰氧基的手性液晶单体(M1～M4),然后再以六氯合铂酸为引发剂,将四种单体通过接枝聚合,获得了对应的聚硅氧烷类液晶高分子(P1～P4),采用FT-IR、1 H-NMR与GPC表征了所合成的中间体、手性液晶单体及其聚合物的化学结构与分子量及分布,结果符合分子设计.此外,采用旋光仪测定了手性单体的旋光度,研究表明:它们均为右旋化合物,其比旋光度随化合物刚性的增加而降低,而对于端基相同、液晶核刚性大小接近的单体,其比旋光度比较接近.     

两类手性PNA单体及其对映异构体的合成

分别以保护的Ｌ－和Ｄ－赖氨酸作为起始原料合成了两种类型的ＰＮＡ单体。在类型Ｉ中，碱基通过－ＣＨ２Ｃ（Ｏ）－间隔臂与赖氨酸的α－ＮＨ相连，而类型Ⅱ中，－Ｃ（Ｏ）－用作连接臂。     

侧基对N-炔丙基酰胺螺旋共聚物光学活性的影响

设计并合成了5个系列的带有不同侧基的手性-非手性N-炔丙基酰胺共聚物,以铑有机配合物为催化剂对单体实施聚合反应得到高产率(>95%)的共聚物,聚合物具有高立构规整性(cis-含量高于94%).利用圆二色(CD)及紫外-可见吸收(UV-Vis)光谱技术对共聚物的二级结构及光学活性进行了表征,当非手性单体的酰胺侧基体积适中时,共聚物具有较高的光学活性,部分共聚物的光学活性甚至高于纯手性聚合物.表明通过选择合适的手性-非手性共聚单体及单体配比,可获得具有高光学活性的螺旋聚合物.     

Enantiomeric separation of chiral peptide nucleic acid monomers by capillary electrophoresis with charged cyclodextrins

Direct chiral separation of chiral peptide nucleic acid (PNA) monomers has been achieved for the first time by capillary electrophoresis (CE) with charged cyclodextrins as chiral selectors added to the electrophoretic buffer. Selectively modified 6-deoxy-6-N-histamino-beta-cyclodextrin and sulfobutyl ether-beta-CD were successfully used as chiral selectors for the enantiomeric separation of chiral monomers based on different aminoethylamino acids bearing thymine or adenine as nucleobases. Chiral separations were obtained at low selector concentrations (1-3 mM) with good enantioselectivity and resolution factors. Separations were optimized as a function of pH in order to exploit the effect of the electrostatic interactions between the oppositely charged selector and selectand. The method has been applied to the analysis of the enantiomeric excess of chiral monomers used for the solid phase synthesis of chiral PNA oligomers. CE chiral analysis showed that a very high enantiomeric purity was generally achieved in the synthesis of all monomers, except for histidine and aspartic acid based monomers in which ca. 10% of the "wrong" enantiomer was always present.     

Efficient and sequence-specific DNA-templated polymerization of peptide nucleic acid aldehydes

On the basis of the distance-dependence of DNA-templated reductive amination reactions and of recent findings of D. Lynn and co-workers, we developed DNA-templated polymerizations of synthetic peptide nucleic acid (PNA) aldehydes. The coupling reactions proceed in a highly efficient and sequence-specific manner, even in the presence of mixtures of PNA aldehydes of different sequence. Synthetic peptide nucleic acid polymers containing as many as 40 PNA units (representing 10 consecutive coupling reactions) were formed efficiently. The ease of preparing PNAs containing tailor-made functional groups together with these findings raises the possibility of evolving synthetic sequence-defined polymers by iterated cycles of translation, selection, PCR amplification, and diversification previously available only to biological macromolecules.     

Synthesis of chiral chromium tricarbonyl labeled thymine PNA monomers via the Ugi reaction

[reaction: see text] Ugi condensation was used to synthesize the first examples of chiral racemic Ar.Cr(CO)(3) labeled peptide nucleic acid (PNA) monomers bearing the organometallic moiety linked to the alpha-carbon of the glycine unit.     

Direct enantiomeric separation of N-aminoethylamino acids: determination of the enantiomeric excess of chiral peptide nucleic acids (PNAs) by GC

Direct chiral separation of N-aminoethylamino acids has been performed for the first time by gas chromatographic (GC) analysis with a Chirasil-Val column, after derivatisation with trifluoroacetic anhydride in dichloromethane, which led to the corresponding piperazin-2-one derivatives, as identified by NMR and GC/MS analysis. The method was used for the analysis of the enantiomeric excess of chiral peptide nucleic acid (PNA) monomers and oligomers after hydrolysis with 6N HCl.     

Aminoethylprolyl peptide nucleic acids (aepPNA): chiral PNA analogues that form highly stable DNA:aepPNA2 triplexes

[formula: see text] The replacement of the glycyl component in the peptide nucleic acid (PNA) backbone by a prolyl unit bearing a nucleobase leads to the aminoethylprolyl (aep) PNAs, which are chiral and cationic. The homooligomeric aepPNA binds to complementary DNA sequences with high affinity and sequence specificity, forming highly stable triplexes.     

Synthesis and photo activity of phenylazonaphthalene peptide nucleic acid monomers

Phenylazonaphthalene peptide nucleic acid （PNA） monomers were successfully synthesized, and their photoisomerization was examined. The new PNA monomers showed reversible trans-cis isomerization with UVand visible light irradiation, which might be the foundation of photo-regulating the hybridization between PNA containing phenylazonaphthalene unit and DNA. Simultaneously, the fluorescence of the new PNA monomers might make them especially useful as structural probes.     

New synthesis of a spin-labeled peptide nucleic acid and its interactions with nucleic acids

A new combined solid-liquid phase synthesis method for a spin labeled peptide nucleic acid (PNA) is developed. The methodology involved initial preparation of a protected PNA on solid phase, followed by efficient solution phase coupling to a spin label containing a reactive carboxylic group. This strategy allows to maintain the integrity of the nitroxide moiety during the various steps of chemical synthesis assuring in the same time the fidelity of the hybridization assay. This compound can be used as a reporter molecule to investigate the binding of peptide nucleic acids to oligonucleotide sequences (DNA or RNA) by EPR spectroscopy.     

Hybridization of pyrrolidinyl peptide nucleic acids and DNA: selectivity, base-pairing specificity, and direction of binding

[structure: see text] A mixed-base, beta-amino acid containing, pyrrolidinyl peptide nucleic acid (PNA) binds strongly and selectively to complementary DNA in an exclusively antiparallel fashion. The PNA-DNA binding specificity strictly follows the Watson-Crick base-pairing rules.     

Direction control in DNA binding of chiral D-lysine-based peptide nucleic acid (PNA) probed by electrospray mass spectrometry

The DNA binding abilities of peptide nucleic acids (PNAs), both achiral and bearing three adjacent D-lysine-based monomers in the middle of the strand ("chiral box" PNA), were studied by means of electrospray mass spectrometry (ESI-MS). In contrast with achiral PNA, "Chiral box" PNA was confirmed to exert high direction control (antiparallel vs. parallel DNA target) in DNA binding.