Ethylation of nucleophilic sites in DNA by N-ethyl-N-nitrosourea depends on chromatin structure and ionic strength

Depending on ionic strength, chromatin can assume either a condensed, supranucleosomal conformation or the form of an extended nucleosomal fiber. Using sedimentation velocity analysis, both types of structures could be identified in chromatin prepared from cell nuclei of fetal rat brain. When the ionic strength was reduced from 60 to 10 mM NaCl, the average S-value of a defined chromatin fiber fraction (12–15 nucleosomes in size) decreased dramatically from 72 S to 55 S, reflecting the unfolding of condensed chromatin to an extended conformation. Correspondingly, the average S-value of histone H1-depleted chromatin (Ch⁻) was 54 S at 60 mM NaCl and did not change significantly at lower NaCl concentrations. Ch⁻ contains only the core histones and is, therefore, relaxed into an extended form.

Using a monoclonal antibody (ER-6) specific for O⁶-ethyldeoxyguanosine, we studied the influence of chromatin conformation on the formation of O⁶-ethylguanine (O⁶-EtGua) in the DNA of chromatin exposed to the carcinogen N-ethyl-N-nitrosourea (EtNU; 1 mg/ml, 37°C, 20 min) in vitro. When the NaCl concentration during incubations with EtNU was varied between 0 and 100 mM, the amount of O⁶-EtGua formed in the DNA of complete chromatin (Ch⁺) was highest at 0 mM NaCl, then decreased exponentially with increasing ionic strength, and remained approximately constant at values 50 mM NaCl. A similar dependence on ionic strength was found for the formation of O⁶-EtGua in the DNA of Ch⁻ and in native DNA. The frequency of O⁶-EtGua was highest in native DNA, followed by the DNA of Ch⁻, and lowest in the DNA of Ch⁺. At each salt concentration, the O⁶-EtGua content of Ch⁺ DNA relative to the corresponding values for Ch⁻ DNA and native DNA, remained unchanged (0.70±0.03 S.D. and 0.42±0.03 S.D., respectively). In addition to O⁶-EtGua, the formation of 7-ethylguanine (7-EtGua; major groove of the DNA double helix) and 3-ethyladenine (3-EtAde; minor groove) was analysed after exposure to [1-¹⁴C]EtNU. 7-EtGua was the most frequently formed ethylation product, followed by O⁶-EtGua and 3-EtAde. As in the case of O⁶-EtGua, the frequencies of 7-EtGua and 3-EtAde were dependent on ionic strength, and decreased in the order: native DNA, Ch⁻ DNA, and Ch⁺ DNA. Compared with native DNA (relative value, 100), the frequencies of O⁶-EtGua and 7-EtGua in DNA were reduced to a similar extent in Ch⁻ (rel. values 62.1 and 61.2, respectively) and in Ch⁺ (rel. values for both products, 43.9). The corresponding values for 3-EtAde were slightly lower in both types of chromatin fibers (rel. values 56.7 and 39.5, respectively). Thus, the core histones generally protect DNA from ethylation by EtNU. While nucleophilic sites in the major groove and in the base-pairing region of the DNA double helix are protected to about the same degree, the N-3 position of adenine in the minor groove is slightly less accessible to the ethyldiazonium ion generated from EtNU. In all cases the highest degree of protection is obtained when histone H1 is present in chromatin.     

A database of 32 DNA triplets to study triple helices by molecular mechanics and dynamics

We present here a database of 32 deoxyribonucleotide triplets, that can be used as building blocks of triple helix forming deoxyribonucleotides on a computer. This database is made of all the pairing schemes of the triplets ATT, GCC⁺, ATA and GCG where the third base forms two hydrogen bonds with the purine of the first two Watson-Crick strands. The essential features of the known triple helices were preserved in the resulting structures. A triple helix can be easily built from any combination of these basic triplets. Four homogeneous and alternate triple helices thus obtained were studied by molecular mechanics and dynamics in vacuo. The results are in agreement with known experimental observations for ATT and suggest a possible structure for the GCG triple helix. In order to characterize the geometry of the structures obtained, the definitions of nucleic acid structure parameters (R.E. Dickerson et al., EMBO J. 8 (1989) 1–4) have been extended to triple helical polynucleotides.     

3nion-independent conformational ordering in iota-carrageenan: Disorder-order equilibria and dynamics

The equilibria and dynamics of the disorder-to-order transition of the anionic polysaccharide iota-carrageenan have been studied in the presence of tetramethyl-ammonium salts. By the use of a stopped-flow polarimeter, the rate equation and temperature dependence of the observed forward rate-constant were found to accord with a co-operative dimerisation process. Activation parameters for helix nucleation were shown to be independent of the anion for solutions containing tetramethylammonium chloride and bromide, i.e., ΔH^‡ = 1 ±3 kJ.mol⁻¹, ΔS^‡ = −178 ±10 J.mol⁻¹.K⁻¹, ΔG^‡_298K = 54 ±2 kJ.mol⁻¹, and k_nuc,298K = 1880 ±80 dm³.mol⁻¹.s⁻¹. The temperature dependence of optical rotation was also shown to be independent of the anion present.     

The infrared absorption of amino acid side chains

Amino acid side chains play fundamental roles in stabilising protein structures and in catalysing enzymatic reactions. These fields are increasingly investigated by infrared spectroscopy at the molecular level. To help the interpretation of the spectra, a review of the infrared absorption of amino acid side chains in H₂O and ²H₂O is given. The spectral region of 2600–900 cm⁻¹ is covered.     

Mg-induced transition to strongly cooperative binding of histone H1 to linear DNA

By addition of Mg²⁺ ions to histone H1-DNA complexes formed at 20mM NaCl a transition to strongly cooperative binding of histone H1 to DNA is induced. In the analytical ultracentrifuge, above a critical Mg²⁺ concentration of about 0.05 mM, the single component representing the original H1-DNA complex is replaced by two components: a higher order H1-DNA complex type characterized by a much higher sedimentation coefficient, and a slow-sedimenting component consisting of essentially H1-free DNA above 0.1 mM Mg^2-. The fast complex diappears upon removal of Mg²⁺, showing that the process is reversible, and also upon addition of urea. Electron microscopy shows the cooperatively formed H1-DNA complexes to appear predominatly as loosely twisted cable rings in unfixed specimens, and as strongly condensed circular structures of different diameter, but approximately uniform thickness (of about 12nm) after fixation with glutaraldehyde. Besides these higher order structures, only single fibres indistinguishable from control DNA may be seen; individual double fibres which, in the absence of Mg²⁺, represent the predominant H1-DNA complexe structure at about 0.4–0.8 w/w H1/DNA are no longer visible. The transition to strongly cooperative binding of H1 occurs at approximately the same Mg²⁺ concentration which is known to induce the folding of the 10 nm nucleosome chain into the 30nm solenoid structure of chromatin.     

Mutations by near-ultraviolet radiation in Escherichia coli strains lacking superoxide dismutase

Om wild-type Escherichia coli, near-ultraviolet radiation (NUV) was only weakly mutagenic. However, in an allelic mutant strain (sodA sodB) that lacks both Mn- and Fe-superoxide dismutase (SOD) and assumed to have excess superoxide anion (O₂⁻), NUV induced a 9-fold increase in mutation above the level that normally occurs in this double mutant. When a sodA sodB double mutant contained a plasmid carrying katG⁺ HP-I catalase), mutation by NUV was reduced to wild-type (sodA⁺ sodB⁺) levels. Also, in the sodA sodB xthA triple mutant, which lacks exonuclease III (exoIII) in addition to SOD, the mutations frequency by NUV was reduced to wild-type levels. This synergistic action of NUV and O₂⁻ suggested that pre-mutational lesions occur, with exoIII converting these lesions to stable mutants. Exposure to H₂O₂ induced a 2.8 fold increase in mutations in sodA sodB double mutants, but was reduced to control levels when a plasmid carrying katG⁺ was introduced. These results suggest that NUV, in addition to its other effects on cells, increases mutations indirectly by increasing the flux of OH^. radicals, possibly by generating excess H₂O₂.     

Effects of calcium binding on the structure and stability of human growth hormone

Thermodynamic analysis of calcium ions binding to human growth hormone (hGH) was done at 27 °C in NaCl solution, 50 mM, using different techniques. The binding isotherm for hGH-Ca²⁺ was obtained by two techniques of ionmetry, using a Ca²⁺-selective membrane electrode, and isothermal titration calorimetry. Results obtained by two ionmetric and calorimetric methods are in good agreement. There is a set of three identical and non-interacting binding sites for calcium ions. The intrinsic dissociation equilibrium constant and the molar enthalpy of binding are 52 μM and −17.4 kJ/mol, respectively. Temperature scanning UV–vis spectroscopy was applied to elucidate the effect of Ca²⁺ binding on the protein stability, and circular dichroism (CD) spectroscopy was used to show the structural change of hGH due to the metal ion interaction. Calcium ions binding increase the protein thermal stability by increasing of the alpha helix content as well as decreasing of both beta and random coil structures.     

Mechanisms of chromosomal aberration production I. Aberration induction by ultraviolet light

We have studied chromosomal aberration production in V-79 Chinese hamster tissue culture cells by UV light administered during the post-DNA-synthetic G₂ phase of the cell cycle. The treatment produced achromatic lesions and some chromatid deletions in the first post-irradiation mitosis, but no isochromatid deletions or chromatid exchange aberrations. In contrast, when G₂ UV-irradiated cells were examined in their second post-irradiation mitosis, there were significant yields of chromatid-type aberrations of all types, including isochromatid deletions and chromatid exchanges.

We have earlier reported²¹ that UV-irradiation during the pre-DNA-synthetic G₁ phase of the cell cycle induces only chromatid aberrations and also that most chromosomal aberration production by UV in G₁ can be photoreactivated in cells possessing the photoreactivating enzyme. We present here a model for chromosomal aberration production by UV. In the model all aberration production is enzymatically mediated, a consequence of the functioning of known molecular repair mechanisms. The important elements in the model are the following:

1. (1) The vertebrate chromosome is mononeme; i.e., contains but a single DNA double helix during the prereplication G₁ phase of the cell cycle.

2. (2) The UV-induced DNA lesion leading to the production of most aberrations is the cyclobutane dimer between adjacent pyrimidines in one polynucleotide strand.

3. (3) Single chain breaks appear at metaphase as achromatic lesions.

4. (4) Dimer removal sometimes leaves unrepaired single chain gaps, possibly as a result of incomplete excision repair.

5. (5) The single-stranded DNA opposite a single chain gap can be cleaved by a single-strand DNAase.

6. (6) Gaps are left in newly synthesized DNA polynucleotide chains opposite defective template chains (i.e., opposite dimers and chain breaks).

7. (7) Double-strand breaks present following local DNA replication may “spread” to the other chromatid by a recombinational process between template and new polynucleotide chains, one from each of the homologous double helices.

The model predicts the occurrence of isoachromatic lesions and of chromatid deletions paired (isolocus) with achromatic lesions. Though often not reported, both do, in fact, occur. In addition, the model accounts for the phenomenon of sister-chromatid exchange as a manifestation of a recombinational, or post-replication, repair mechanism. Finally, the model offers a simple interpretation of chromosomal aberration production by a variety of chemical agents.     

Influence of magnesium ions on biofilm formation by Pseudomonas fluorescens

Mg²⁺ can potentially influence bacterial adhesion directly through effects on electrostatic interactions and indirectly by affecting physiology-dependent attachment processes. However, the effects of Mg²⁺ on biofilm structure are largely unknown. In this study, Pseudomonas fluorescens was used to investigate the influence of Mg²⁺ concentration (0, 0.1 and 1.0 mM MgCl₂) on biofilm growth. Planktonic and attached cells were enumerated (based on DAPI staining) while biofilm structures were examined via confocal laser scanning microscopy and three-dimensional structures were reconstructed. Mg²⁺ concentration had no influence on growth of planktonic cells but, during biofilm formation, Mg²⁺ increased the abundance of attached cells. For attached cells, the influence of Mg²⁺ concentration changed over time, suggesting that the role of Mg²⁺ in bacterial attachment is complex and dynamic. Biofilm structures were heterogeneous and surface colonization and depth increased with increasing Mg²⁺ concentrations. Overall, for P. fluorescens, Mg²⁺ increased initial attachment and altered subsequent biofilm formation and structure.     

长期不同施肥模式对南方双季稻田生态系统净碳汇效应和经济收益的影响

施肥措施与稻田生态系统净碳汇效应、经济收益的关系密切。本研究以长期(35年)定位施肥试验田为平台,分析了单独施用化肥(MF)、秸秆还田+化肥(RF)、30%有机肥+70%化肥(OM)和无肥对照(CK)4种不同施肥模式对我国南方双季稻田耕层土壤固碳速率、碳密度、年碳汇平衡和经济收益的影响。研究表明: 不同施肥处理双季稻田耕层土壤碳库变化范围为216.02～866.74 kg·hm^-2·a^-1,OM处理土壤碳年变化量显著高于MF、RF和CK处理;双季稻田土壤固碳速率为51.5～650.7 kg·hm^-2·a^-1,表土碳密度为55.64～78.42 t·hm^-2,各施肥处理高低顺序均为OM>RF>MF>CK。各施肥处理双季稻田生态系统水稻的碳吸收为4.42～9.32 t C·hm^-2·a^-1,其高低顺序为OM>RF>MF>CK;与MF处理相比,OM和RF处理稻田土壤净碳汇量分别提高了27.6%和13.6%。各施肥处理双季稻田生态系统的碳成本物质投入变化范围为1.49～2.17 t C·hm^-2·a^-1,年经济收益变化范围为1.30×10³～7.83×10³元·hm^-2·a^-1,其高低顺序为RF>OM>MF>CK;OM、RF和MF处理双季稻田生态系统经济效益的净收益均显著高于CK处理。总之,长期施用有机肥、秸秆还田配施化肥措施均有利于增加双季稻田土壤固碳速率、碳汇效应和经济收益,是提高南方双季稻田土壤有机碳贮量的施肥模式。     

Structure of [Ni(dippe)(μ-S)]2 and its reaction products. The nucleophilicity of the Ni2S2 fragment

The dimer [(dippe)Ni(μ-S)]₂ reacts with organic electrophiles to give the alkylated species [(dippe)₂Ni₂(μ-S)(μ-SR)]⁺. Stronger alkylating agents lead to double alkylation and cleavage of the dimer. Protonation similarly occurs with strong acids. The structures of several of these species have been determined.     

Identification of Residues in Transmembrane Regions III and VI that Contribute to the Ligand Binding Site of the Serotonin 5-HT6 Receptor

Abstract: We have examined the ligand binding site of the serotonin 5-HT₆ receptor using site-directed mutagenesis. Replacing the highly conserved Asp¹⁰⁶ in transmembrane region III by asparagine eliminated d -[³H]lysergic acid diethylamide ([³H]LSD) binding to the mutant receptor transiently expressed in HEK293 cells. The potency of 5-HT and LSD to stimulate adenylyl cyclase was reduced by 3,600- and 500-fold, respectively, suggesting that an ionic interaction between the positively charged amino group of 5-HT and D106 is essential for high-affinity binding and important for receptor activation. In addition, basal cyclic AMP levels in cells expressing this mutant were increased. Mutation of a tryptophan residue one helix turn toward the extracellular side of transmembrane region III (Trp¹⁰²) to phenylalanine produced significant changes in the binding affinity and potency of several ligands, consistent with a role of this residue in the formation of the ligand binding site. The exchange of two neighboring residues in the carboxy-terminal half of transmembrane region VI (Ala²⁸⁷ and Asn²⁸⁸) for leucine and serine resulted in a mutant receptor with increased affinities (seven- to 30-fold) for sumatriptan and several ergopeptine ligands. The identification of these interactions will help to improve models of the 5-HT₆ receptor ligand binding site.     

旱地全膜双垄沟玉米生产的AquaCrop模型模拟及管理措施优化

为研究AquaCrop模型模拟旱地全膜双垄沟栽培模式的适用性,寻求最佳农艺管理措施,本研究选择2014和2015年玉米施氮梯度试验数据对模型中品种和胁迫参数进行率定和验证,并模拟不同管理措施水平下产量变化趋势.结果表明: 所有处理实测和模拟产量的平均根方误差(RMSE)、标准化均方根误差(NRMSE)和符合度指数(d)分别为717 kg·hm^-2、10.0%和0.96,总生物量的RMSE、NRMSE和d分别为951 kg·hm^-2、6.5%和0.98,能够较好的反映旱地全膜双垄沟玉米的栽培特性;在冠层覆盖度和生物量动态模拟分析中得出施氮270 kg N·hm^-2时的拟合度最好,随着氮肥的胁迫增加,模拟精度逐渐降低;甘肃中部地区全膜双垄沟玉米栽培模式中最佳播种期在4月下旬至5月上旬,播种密度为45000～65000株·hm^-2,生育期时长在130～145 d,施氮量为240～280 kg·hm^-2.本研究结果对AcquaCrop模型在甘肃干旱区域的应用具有一定参考价值,而且有助于农业栽培技术的转化和推广.     

气候变化对广东省双季稻种植气候区划的影响

基于广东省86个气象站1961—2016年的气温资料和1∶25万数字高程模型(DEM)数据,采用线性趋势分析、累积距平和反距离权重插值等方法,分析影响双季稻种植的关键气候因子(双季稻安全生育期日数、≥10 ℃积温)时空变化特征,结合气候因子在1961—1990年、1971—2000年、1981—2010年、气候因子突变前(1961—1997年)、突变后(1998—2016年)等5个时间段的变化,研究了气候变化对广东双季稻熟性搭配分布区域及其面积的影响.结果表明: 广东省双季稻安全生育期日数、≥10 ℃积温的空间分布表现为南高北低、平原高山区低.近56年,广东双季稻安全生育期日数以1.7 d ·10 a^-1的速率显著增加,≥10 ℃积温以43 ℃·d·10 a^-1的速率显著上升,各气候因子均在1997年发生了突变.广东双季稻熟性搭配可分为早熟+早熟、早熟+晚熟和晚熟+晚熟3个气候区.早熟+早熟区主要分布在北部中亚热带地区,早熟+晚熟区主要分布在中部南亚热带地区,晚熟+晚熟区主要分布在南部北热带地区.受气候变化的影响,广东晚熟+晚熟区面积明显扩大,早熟+晚熟区面积明显减小,而早熟+早熟区的面积变化不明显.与1961—1990年相比,1971—2000年和1981—2010年广东省晚熟+晚熟区面积分别增加了1.22×10⁶和2.56×10⁶ hm²,早熟+晚熟区的面积分别减小了1.13×10⁶和2.56×10⁶ hm².与突变前(1961—1997年)相比,突变后(1998—2016年)晚熟+晚熟区的面积增大一倍多,早熟+晚熟区面积缩小近一倍.     

Natural competence in strains of Actinobacillus pleuropneumoniae

The fatty acid (FA) profiles of myxobacteria contain FA species with double bonds at the Δ⁵ and Δ¹¹ positions, the latter being rather unusual among bacteria. Despite this knowledge, the mechanism for introduction of these double bonds has never been described before in myxobacteria. Searches for candidate genes in the genome of the model organism Myxococcus xanthus revealed 16 genes, which have been annotated as FA desaturases. However, due to redundant substrate specificity, functional analyses of these enzymes by construction of inactivation mutants did not lead to the identification of their function or substrate specificity. Therefore, we elucidated the regioselectivity of the desaturation reactions by heterologous expression of eight desaturases from M. xanthus in Pseudomonas putida and thus could prove five of them to be indeed active as desaturases, with three (MXAN_1742, MXAN_3495 and MXAN_5461) and two (MXAN_0317 and MXAN_6306) acting as Δ⁵ and Δ¹¹ desaturases, respectively. This is the first report about the heterologous expression and regioselectivity of FA desaturases in myxobacteria.     

Mechanisms of chromosomal aberration production II. Aberrations induced by 5-bromodeoxyuridine and visible light

We have allowed synchronized V79B Chinese hamster tissue culture cells to incorporate 5-bromodeoxyuridine (BUdR) during one DNA synthetic (S) period of the cell cycle and then determined chromosomal aberration yields induced by illumination of the cells with visible light during the succeeding pre- and post-DNA-synthetic (G₁and G₂) phases of the cell cycle. At the level used, BUdR by itself induces no aberrations. Illumination during the G₁ phase following incorporation induces aberrations of the chromatid type, but none of the chromosome type. All types of chromatid aberrations are induced, including isochromatid deletions and exchange types. In contrast, when cells are illuminated during the immediately following G₂ phase, large numbers of achromatic lesions and chromatic deletions are seen at the first post-illumination mitosis, but no isochromatid deletions and few exchange-type aberrations occur. When G₂-illuminated cells are examined in their second mitosis, however, chromatid aberrations of all types are again seen.

These results are interpreted within the “repair” model of chromosomal aberration production by UV light presented earlier³. The model assumes that the vertebrate chromosome is mononeme, consisting of but a single DNA double helix during the prereplication G₁ phase. The initial lesions induced by illumination of BUdR-containing DNA are believed to be single-chain breaks, and the observation that G₁ illumination produces only chromatid-type aberrations is taken as additional evidence for the mononeme chromosome. Conversion of single-chain breaks into double chain breaks through the action of a single-strand nuclease is postulated to account for the production of chromatid deletions at the first mitosis of G₂-illuminated cells. The action of this enzyme, plus a recombinational or post-replication repair mechanism, are postulated to account for the production of isochromatid deletions in G₁-illuminated cells. A rapid decline in achromatic lesion frequency with increasing time between G₂ illumination and fixation of the cells is considered evidence for rapid rejoining of most of the initial chain breaks.     

Kinetics and equilibria of Ga(III)---thiocyanate complex formation. Mechanism of ligand substitution reactions of Ga(III) in aqueous solution

The kinetics and equilibria of complex formation by Ga(III) with NCS⁻ in aqueous solution have been measured over a range of acidities and temperatures, the contributing paths to the reaction resolved, and their rate constants and activation parameters determined. The hydrolysis equilibria required to carry out this resolution of kinetic behaviour have also been measured.

Unlike the other reported complexation reactions of Ga(III) in aqueous solution, the separate reaction pathways can be assigned with no ambiguity. At 25 °C and ionic strength 0.5 M, the observed forward rate constant for the complex formation is described by {k₁ + k₂K_1h/[H⁺] + k₃K_1hK_2h/[H⁺]²} M⁻¹ s⁻¹. For these conditions, the first and second successive hydrolysis constants of Ga(H₂O)₆³⁺ are given by pK_1h = 3.69 ± 0.01 and pK_2h = 3.74 ± 0.04. The rate constants corresponding to the reactions of the species Ga(H₂O)₆³⁺, Ga(H₂O)₅(OH)²⁺ and Ga(H₂O)₄(OH)₂⁺ with NCS⁻ are k₁ = 57 ± 4 M^{−1 −1}, k₂ = (1.08 ± 0.01) × 10⁵ M⁻¹ s⁻¹ and k₃ = 3 × 10⁶ M⁻¹ s⁻¹ respectively. The complexation equilibrium quotient [GaNCS²⁺]/([Ga³⁺][NCS⁻]) has been independently determined by spectrophotometric titration to be 20.8 ± 0.3 M⁻¹ at 25 °C and ionic strength 0.5 M.

These kinetic results lead to an interpretation of the data, and a reinterpretation of other data for aquo-Ga(III) complex formation kinetics from the literature which support the assignment of a dissociative interchange mechanism for these reactions rather than the associative activation mode sometimes proposed.     

Asn229 in the third helix of VPAC1 receptor is essential for receptor activation but not for receptor phosphorylation and internalization: comparison with Asn216 in VPAC2 receptor

After stimulation with agonist, G protein coupled receptors (GPCR) undergo conformational changes that allow activation of G proteins to transduce the signal, followed by phosphorylation by kinases and arrestin binding to promote receptor internalization. Actual paradigm, based on a study of GPCR-A/rhodopsin family, suggests that a network of interactions between conserved residues located in transmembrane (TM) domains (mainly TM3, TM6 and TM7) is involved in the molecular switch leading to GPCR activation.

We evaluated in CHO cells expressing the VPAC₁ receptor the role of the third transmembrane helix in agonist signalling by point mutation into Ala of the residues highly conserved in the secretin-family of receptors: Y²²⁴, N²²⁹, F²³⁰, W²³², E²³⁶, G²³⁷, Y²³⁹, L²⁴⁰. N²²⁹A VPAC₁ mutant was characterized by a decrease in both potency and efficacy of VIP stimulated adenylate cyclase activity, by the absence of agonist stimulated [Ca²⁺]_i increase, by a preserved receptor recognition of agonists and antagonist and by a preserved sensitivity to GTP suggesting the importance of that residue for efficient G protein activation. N²²⁹D mutant was not expressed at the membrane, and the N²²⁹Q with a conserved mutation was less affected than the A mutant. Agonist stimulated phosphorylation and internalization of N²²⁹A and N²²⁹Q VPAC₁ were unaffected. However, the re-expression of internalized mutant receptors, but not that of the wild type receptor, was rapidly reversed after VIP washing. Receptor phosphorylation, internalization and re-expression may be thus dissociated from G protein activation and linked to another active conformation that may influence its trafficking.

Mutation of that conserved amino acid in VPAC₂ could be investigated only by a conservative mutation (N²¹⁶Q) and led to a receptor with a low VIP stimulation of adenylate cyclase, receptor phosphorylation and internalization. This indicated the importance of the conserved N residue in the TM3 of that family of receptors.