γ-Ray-Radiation-Scissioned Chitosan as a Gene Carrier and Its Improved in vitro Gene Transfection Performance

Chitosan （CS） is expected to be an ideal gene carrier for its high biosafety. In this work, CS with low molecular weight were prepared through the γ-ray radiation on the acetic acid solution of CS. The CS chains were scissioned under the γ-ray radiation, and the molecu- lar weight （MW） of CS decreased with the absorbed dose. When the absorbed dose was above 30 kGy, the molecular weight of CS decreased about an order of magnitude. The γ-ray-radiation-scissioned CS can effectively bind with plasmid （pEGFP） through complex coacervation method, forming pEGFP/γ-ray-radiation-scissioned CS complex particles with a size of 200-300 nm. The complex particles have good stability and little cytotoxicity. The in vitro gene transfection efficiencies of the pEGFP/γ-ray-radiation-scissioned CS complex particles were investigated by fluorescence microscope and flow cytometry. The results showed that the gene vectors using γ-ray-radiation-scissioned CS as the carrier will possess better gene transfection efficiency than those using natural high-MW CS as the carrier. The higher the absorbed dose, the smaller the MW of CS and the better transfection efficiency of the corresponding gene vector. This work provides a green and simple method on the preparation of CS-based gene vectors with high efficiency and biosafety.

Gene expression arrays as a tool to unravel mechanisms of normal tissue radiation injury and prediction of response

Over the past 5 years there has been a rapid increase in the use of microarray technology in the field of cancer research, The majority of studies use microarray analysis of tumor biopsies for profiling of molecular characteristics in an attempt to produce robust classifiers for prognosis. There are now several published gene sets that have been shown to predict for aggressive forms of breast cancer, where patients are most likely to benefit from adjuvant chemotherapy and tumors most likely to develop distant metastases, or be resistant to treatment. The number of publications relating to the use of microarrays for analysis of normal tissue damage, after cancer treatment or genotoxic exposure, is much more limited. A PublVled literature search was conducted using the following keywords and combination of terms： radiation, normal tissue, microarray, gene expression profiling, prediction. With respect to normal tissue radiation injury, microarrays have been used in three ways： （1） to generate gene signatures to identify sensitive and resistant populations （prognosis）; （2） to identify sets of biomarker genes for estimating radiation exposure, either accidental or as a result of terrorist attack （diagnosis）; （3） to identify genes and pathways involved in tissue response to injury （mechanistic）. In this article we will review all （relevant） papers that covered our literature search criteria on microarray technology as it has been applied to normal tissue radiation biology and discuss how successful this has been in defining predisposition markers for radiation sensitivity or how it has helped us to unravel molecular mechanisms leading to acute and late tissue toxicity. We also discuss some of the problems and limitations in application and interpretation of such data.

Identification and Validation of Candidate Radiation-responsive Genes for Human Biodosimetry

The aim of the present study is to analyze the global research trend of radiation-responsive genes and identify the highly reproducible radiation-responsive genes. Bibliometric methods were applied to analyze the global research trend of radiation-responsive genes. We found 79 publications on radiation-responsive genes from 2000 to 2017. A total of 35 highly reproducible radiation-responsive genes were identified. Most genes are involved in response to DNA damage, cell proliferation, cell cycle regulation, and DNA repair.The p53 signal pathway was the top enriched pathway. The expression levels of 18 genes in human B lymphoblastoid cell line（AHH-1） cells were significantly up-regulated in a dose-dependent manner at 24 h after exposure to 0-5 Gy ^60 Coγ-ray irradiation. Our results indicate that developing a gene expression panel with the 35 high reproducibility radiation-responsive genes may be necessary for qualitative and quantitative assessment after exposure.

Radiation and androgen withdrawal alter expression of apoptosis pathway genes of prostate cancer cells

Aim: To investigate the altered expression of apoptosis pathway genes of prostate cancer cells treated by radiation and androgen withdrawal and whether the combined treatment may induce additive apoptosis. Methods: Androgen sensitive prostate cancer cell line LNCaP was cultured and treated by radiation, androgen withdrawal and combination of the two. Apoptosis was determined using apoptotic cells staining and mononuclear cell direct cytotox-icity assay. The total RNA were extracted and harvested. cDNA probes were prepared and labeled with biotin-16-dUTP and then hybridized to commercially available cDNA arrays, including apoptosis pathway-specific genes. The expression of important gene was further determined using RT-PCR. Results: Radiation induced additive apoptosis of prostate cancer cells; androgen withdrawal exhibited synergetic action. TNFRSF8 variant 2, DFFA, LTbR, mdm2, Myd88, TNFRSF14 and TNFSF4 mRNA were up regulated by radiation, while Survivin and Bar mRNA were down regulated. Mcl-1, TNFRSF14, MyD88 and TNFSF4 mRNA were up regulated by androgen withdrawal, while Bar, Survivin and TRAIL-R3 mRNA were down regulated. Conclusion: Radiation and androgen withdrawal altered the expression of apoptosis pathway genes of prostate cancer cells in different patterns, which may contribute to the additive apoptotic effect induced by the combined treatment.

EXPRESSION AND CLINICAL SIGNIFICANCE OF MULTIDRUG RESISTANCE GENE AND MULTIDRUG RESISTANCE-ASSOCIATEDPROTEIN GENE IN ACUTE LEUKEMIA

Objective: To evaluate the expression and clinical significance of multidrug resistance gene (mdr1) and multidrug resistance-associated protein (MRP) gene in acute leukemia. Methods: The expression of mdr1 and MRP assay in 55 patients with acute leukemia (AL) by reverse transcription polymerase chain reaction (RT-PCR). Results: The mdr1 and MRP gene expression levels in the relapsed AL and the blastic plastic phases of CML were significantly higher than those in the newly diagnostic AL and controls. The mdr1 and MRP gene expression levels in the clinical drug-resistant group were significantly higher than those in the non-drug-resistant group. The complete remission (CR) rate in patients with high mdr1 expression (14.3%) was significantly lower than that with low mdr1 expression (57.5%); similarly the CR rate in patients with high MRP level was also lower than that with low MRP level. Using both high expression of mdr1 and MRP gene as the indicator for evaluating multidrug resistance (MDR), the positive predictive value and accuracy increased in comparison with single gene high expression. Conclusion: Elevated level of mdr1 or MRP gene expression might be unfavorable prognostic factors for AL patient and may be used as an important index for predicting drug-resistance and relapse in AL patient. Measuring both mdr1 and MRP gene expression would increase accuracy and sensibility of evaluating MDR in acute leukemia.

Science Letters:Assignment of CCR7 gene to chicken chromosome 27 by radiation hybrid panel mapping

The protein encoded by CC chemokine receptor 7 (CCR7) is a member of the G protein-coupled receptor family. This receptor was identified as a gene induced by the Epstein-Barr virus (EBV), and is thought to be a mediator of EBV effects on B lymphocytes. This receptor is expressed in various lymphoid tissues and activates B and T lymphocytes. It has been shown to control the migration of memory T cells to inflamed tissues, as well as stimulate dendritic cell maturation. To map the CCR7 gene in chicken chromosome, a 6 000 rads chicken-hamster radiation hybrid panel (ChickRH6) was used. PCR of samples from ChickRH6 revealed that the location of CCR7 gene is linked to the maker SEQ0347 (6 cR away) with LOD score of 16.6 and that the marker SEQ0347 is located on chromosome 27 at 27 cR of RH (radiation hydrid) map. We compared the corresponding human mRNA sequence with the predicted coding sequence of chicken CCR7 gene, and found that the assembled contig shared a high percentage of similarity with that of the human gene.

MOLECULAR ANALYSIS OF RADIATION-INDUCED MUTATION IN EXON 7/8 OF RAT HPRT GENE

Objective To investigate the relationship between the radiation dose and the HPRT gene lo-cus mutation in rat smooth muscle cells, and provide the molecular basis for prevention of restenosis after percutaneous transluminal coronary angioplasty (PTC4). Methods The smooth muscle cells cultured in vitro were irradiated by radionuclide 188Re in different doses. HPRT gene mutation colonies were selected and isolatedby 6-thioguanine. Analysis of mutation in exon 7/8 of HPRT gene were accomplished by polymerase chain reaction and single-strand conformation polymorphism. Results The HPRT gene mutation frequency of rat smooth muscle cells that were irradiated by radionuclide 188Re ranged from 5.5× 10-6 to 13 ×10-6. Of 91 HPRT gene mutation colonies, 13 (14.3%) contained exon 7/8 deletion and 15(16.5%) had point mutation.The exon 7/8 mutation frequency was 30.8% . There were significant relationships between radiation dose and mutation frequency of HPRT gene and exon 7/8 . Conclusion The DNA damage and gene mutation inducedby radiation has positive relationship with radiation dose, and is a basis of proliferation inhibition and apopto-sis of smooth muscle cells.

Mechanism of exogenous nucleic acids and their precursors improving the repair of intestinal epithelium after 7-irradiation in mice

AIM To clone expressed genes associated withrepair of irradiation-damaged mice intestinalgland cells treated by small intestinal RNA,andto explore the molecular mechanism ofexogenous nucleic acids improving repair ofintestinal crypt.METHODS The animal mode of test group andcontrol group was established,forty-five micebeing irradiated by γ ray were treated with smallintestinal RNA as test group,forty mice beingirradiated by γ ray were treated withphysiological saline as control group,five micewithout irradiation were used as normal control,their jejunal specimens were collectedrespectively at 6h,12h,24h,4d and 8d afterirradiation.Then by using LD-PCR based onsubtractive hybridization,these gene fragmentsdifferentially expressed between test group andcontrol group were obtained,and then werecloned into T vectors as well as beingsequenced.Obtained sequences were screenedagainst.GeneBank,if being new sequences,they were submitted to GeneBank.RESULTS Ninety clones were associated withrepair of irradiation-damaged intestinal glandcells treated by intestinal RNA.These clonesfrom test group of 6h,12h,24h,4d and 8dwere respectively 18,22,25,13,12.By screening against GeneBank,18 of which werenew sequences,the others were dramaticallysimilar to the known sequences,mainly similarto hsp,Nmi,Dutt1,alkaline phosphatase,homeobox,anti-CEA ScFv antibody,arginine/serine kinase and BMP-4,repA.Eighteen genefragments were new sequences,their acceptnumbers in GeneBank were respectivelyAF240164-AF240181.CONCLUSION Ninety clones were obtained tobe associated with repair of irradiation-damagedmice intestinal gland cells treated by smallintestinal RNA,which may be related toabnormal expression of genes and matchedproteins of hsp,Nmi,Duttl,Na,K-ATPase,alkalineph-osphatase,glkA,single strandedreplicative centromeric gene as well as 18 newsequences.

RADIATION-INDUCED APOPTOSIS OF TWO NASOPHARANGEALCARCINOMA CELL LINES

Objective: To study apoptosis induced by radiation in two nasopharyngeal carcinoma (NPC) cell lines, CNE and CNE-2. Methods: Hoechst 33342 staining, immuno-histochemical staining, RT-PCR, DNA dot blotting and Southern blotting were used to identify apoptosis. Results: A single dose of X-irradiation resulted in apoptosis, the apoptotic index (AI) was time- and dose-dependent. Different apoptotic responses existed in the two cell lines. Immunohistochemical staining showed that bcl-2 protein was strongly positive in CNE but negative in CNE-2. However, RT-PCR revealed p53 mRNA in CNE-2 but not in CNE. P53 and bcl-2 genes were both present in the two cell lines as shown by DNA blotting, but the 2.8 kb fragment of the p53 gene was much lower than the 5.6 kb fragment on CNE which was clearly shown in Southern hybridization, suggestive of partial deletion of p53 gene in CNE. Conclusion: Apoptotic response to radiation is different in two NPC cell lines. CNE is more radioresistant than CNE-2. Overexpression of bcl-2 protein and partial deletion of p53 gene may explain their difference in radiosensitivity.

Study on the Protective Effects of Compound Blood-activating Soup on Bone Marrow Hematopoietic Cells in Acute Radiation Injured Mice

After irradiation with 8 Gy 60Coγ-ray,mice were immediaterly given intraperitoneal injection of 200 mg 100 % compound blood-activating soup twice a day. On the 3rd and 7th day, the P53 gene expression of bone marrow hematopoietic cells in Chinese drug group was found to be higher than that in normal group, and it was also significantly higher than that in control group. The expression level of GADD153 gene which was not expressed in normal group was much lower in Chinese drug group than that in control group. On the 7th day after irradiation, the P53 and GADD153 gene expression levels of splenic mononuclear cells were consistent with those of bone marrow hematopoietic cells both in Chinese drug group and control group. On the 3rd and 7th day, the bone marrow hematopoietic tissue volume in Chinese drug group was higher than that in control group, with no difference found between the two groups. While on the 14th day, the difference became significant (P＜0. 01). The results showed that commonly used blood-activating and stasis-eliminating drugs may strengthen .the viability of hematopoietic cells and promote the rehabilitation of hematopoiesis by inducing wt-P53 expression to block the bone marrow hematopoietic cells in G1 phase, during which DNA could be repaired.

Apoptotic Sensitivity to Irradiation Increased after Transfection of chk1 Antisense Chain to HL-60 Cell Line

Summary： The HL-60 cells were transfected with chkl antisense and sense chain, and 24 h later subjected to irradiation. Twenty-four h after irradiation, the changes in the chk1 protein expression was assayed by Western blot, and the cell cycles and apoptosis rate detected by FCM. The irradiated apoptosis sensitivity was increased by antisense blocking of chk1 gene in HL-60 cell line with the apoptosis rate being 26.31 %, significantly higher than that by the sense blocking （10.34 %, 0. 025〈P〈0.05）. In HL-60 cells transfected with chkl antisense chain, the G2/M phase arrest was attenua：ted and the cells in G2/M phase were accounted for 38.42 %, significantly lower than those of the cells transfected with chkl sense chain （54.64 %, 0. 005〈P〈0.01）. It was concluded that antisense blocking of chk1 gene could increase the apoptosis sensitivity to irradiation.

Changes in Gene Expression in Needles and Stems of Pinus radiata Rootstock Plants of Different Ontogenic Age

A major problem in forest clonal productivity is the loss of morphogenetic capability with the increasing age of plants. However, despite of the importance of loss of morphogenetic competence, very little research has been done about the underlying mechanisms involved in this process. For this reason, a gene expression analysis using dot blot technique was performed in needles and stems of 1- and 3-year old Pinus radiata rootstock plants with a proved decrease in morphogenetic competence. Needles of one year old rootstock plants showed a higher number of up-regulated in genes mainly corresponding to photosynthesis and protein synthesis, degradation and modification, reflecting a higher number of active pathways in younger hedges, contrary to the older ones. Gene expression profiles found in stems are in agreement with those found in needles, indicating more active pathways in younger rootstock plants than in older ones. Several transcripts regulating transcription and translation were up-regulated in young competent tissues. Three-year-old stems presented an increase in the expression of an ethylene response factor, involved in plant organ senescence, indicating that pathways involved in senescence and ageing might inhibit the adventitious root formation, as in the older cuttings.

Effect of rhBMP-2m on c-Myb gene expression in bone marrow of irradiated mice

Objective:To exploretheexpressionof c-Mybgenein thebonemarrowcellof irradiatedmicetreated with rhBMP-2manditssignificance.Methods:By wayof RT-PCRandRNAdotblot,we observedtheexpressionof c-Myb geneinthebonemarrowcellsof micetreateddifferentlyon day10andday20afterirradiationrespectively.Results:On day10afterirradiation,theexpressionof c-Mybgeneinthebonemarrowcellof irradiatedmicetreatedwithrhBMP-2mis evidentlyhigherthanthatinnormalmice,andalsohigherthanthatonlytreated withirradiation.However,on day20after irradiation,thereareno evidentdifferencesin thethreegroups.Con clusion:c-Mybgenetakespartin therecoveryof hematopoiesisduringthestageof acuterecoveryinbonemarrow afterirradiation,andtheeffectis enhancedinthepartici-pationof rhBMP-2m.

Radioprotective effects of the expression of FLT3 ligand regulated by Egr-1 regulated element on radiation injury of SCID mice

Objective: In order to explore the radioprotective effects of the expression of hematopoietic growth factors regulated by radio-inducible promoter on radiation injury. Methods:The human FL (Flt3 ligand) cDNA and EGFP (enhanced green fluorescent protein) cDNA were linked together with IRES and then inserted into the eukaryotic expression vector pCI-Egr, which was constructed by substituting CMV promoter in pCIneo with the Egr-1 promoter (Egr-EF). The vector was transferred into human bone marrow stromal ...

沉默GOLM1对宫颈癌Siha细胞放射敏感性影响和机制研究

目的:研究GOLM1对人宫颈癌Siha细胞放射敏感性影响和可能机制。方法:构建慢病毒载体敲低宫颈癌细胞Siha中GOLM1的表达,qPCR检测干扰效率。采用4 Gy X线照射细胞后利用MTT实验检测细胞活性。将经射线照射后的宫颈癌细胞分为GOLM1-SiRNA组、NC-SiRNA组、GOLM1-SiRNA联合IGF1组,观察细胞形态,细胞侵袭和迁移实验观察侵袭和迁移能力,克隆形成实验检测细胞增殖能力。Western blot检测上皮间充质转化相关蛋白及PI3K/Akt通路蛋白。结果:经射线照射后,敲低Siha细胞中GOLM1表达组细胞活性下降最明显,细胞侵袭能力、迁移能力降低,克隆形成能力下降。GOLM1-SiRNA联合PI3K/Akt信号转导通路激活剂IGF1组细胞侵袭、迁移能力增加,克隆形成能力增强。降低GOLM1的表达增强了上皮标记蛋白E-cadherin的表达,同时降低了间质标记蛋白N-cadherin和p-Akt的表达,加入IGF1后E-cadherin蛋白的表达降低,N-cadherin和p-Akt蛋白的表达增强。结论:GOLM1表达降低增加了射线照射后宫颈癌细胞对放射线的敏感性。该作用可能通过介导PI3K/Akt信号转导通路影响细胞的侵袭及迁移能力实现的。

复方斑蝥胶囊联合旋转容积调强技术对头颈部放疗生存期及血清XRCC1、XRCC3mRNA水平的影响

目的探究复方斑蝥胶囊联合旋转容积调强技术对头颈部放疗患者生存期及血清X线修复交错互补基因1(X-ray Repair Cross Complementing 1,XRCC1)、X线修复交错互补基因3(X-ray Repair Cross Complementing 3,XRCC3)信使核糖核酸(Messenger RNA,mRNA)水平的影响。方法选取2019年6月—2021年7月医院收治的头颈部肿瘤患者97例作为研究对象,根据治疗方法不同进行分组,对照组(48例)采用旋转容积调强技术结合放疗治疗,联合组(49例)在对照组基础上加用复方斑蝥胶囊治疗。观察比较临床疗效、中医证候积分、血清XRCC1及XRCC3mRNA水平、生存期、不良反应。结果联合组客观缓解率高于对照组(P<0.05),但疾病控制率与对照组比较差异无统计学意义(P>0.05)。联合组自汗、恶心呕吐、神疲乏力、食欲差、失眠、头晕眼花等得分低于对照组(P<0.05)。联合组血清XRCC1、XRCC3水平及外周血XRCC1、XRCC3 mRNA表达均低于对照组(P<0.05)。联合组无进展生存期和总生存期均高于对照组(P<0.05)。联合组不良反应发生率(34.69%,17/49)低于对照组不良反应发生率(72.92%,35/48)(P<0.05)。结论复方斑蝥胶囊联合旋转容积调强技术能改善头颈部放疗患者肿瘤客观缓解率,缓解临床症状,降低血清XRCC1、XRCC3mRNA水平,减少不良反应。

基于生信分析放射性肺损伤核心基因及靶向中药筛选

为了探索放射性肺损伤发病机制及预测潜在靶向治疗的中药,利用生物信息学方法分析放射性肺损伤与正常肺组织的表达差异基因,从GEO数据库选取GSE202586数据集,通过GEO_(2)R分析得出表达差异基因,对表达差异基因进行GO功能富集分析及KEGG信号通路分析,通过STRING数据库构建蛋白互作网络,利用Cytoscape获得核心基因,通过Coremine Medical预测靶向作用于核心基因的中药.结果共获得差异基因113个,其中88个基因表达上调,25个基因表达下调,主要涉及细胞过程、免疫过程及信号的调节,非跨膜蛋白酪氨酸激酶和信号受体的活性等生物过程;主要富集在免疫系统信号通路.蛋白互作分析筛选出8个核心基因包括CD19,CD22,CD52,CD86,LCP2,PAX5,SPN,TNFRSF13C.将筛选整合得到的8个核心基因通过数据库进行靶向中药的筛选,归纳总结3类相关治疗的中药,包括以赤芍、苦蘵、白花蛇钱草、白英为代表的清热解毒药,以槐角、姜黄、川牛膝为代表的凉血止血、活血化瘀药,以枳实、车前子、灵芝、野山药为代表的补气理气药.该研究利用生物信息学分析预测放射性肺损伤发生的作用机制及潜在治疗的中药,为进一步的科学研究与临床应用提供参考.

DNA损伤效应主动监测的抗氧化基因缺失微生物传感器的构建及性能评价

目的活性氧基团(ROS)水平升高会引起生物体的DNA氧化损伤,监测DNA的氧化损伤程度,能够实现ROS损伤效应的有效评价。基于微生物传感器监测DNA损伤效应可以定量评价氧化损伤程度,但微生物本身具有的ROS清除机制,会影响监测灵敏度。本研究旨在敲除细菌ROS清除机制的关键基因,构建抗氧化基因缺失微生物传感器,实现对DNA损伤效应的灵敏监测,评价ROS对生物体的损伤效应。方法本研究基于λ-Red同源重组的方法敲除细菌抗氧化损伤相关基因ahpCF、katE与katG,构建抗氧化基因缺失微生物传感器,并评价传感器对萘啶酮酸钠和紫外照射的响应。结果成功构建ΔahpCF、ΔahpCF/ΔkatE与ΔahpCF/ΔkatE/ΔkatG三种抗氧化基因缺失的微生物传感器,工程菌ΔahpCF/ΔkatE/ΔkatG对DNA损伤试剂萘啶酮酸钠的响应灵敏度最高,检测限为0.40μmol/L,另外,1.80 min的紫外照射(254 nm)可诱导工程菌产生显著的荧光表达效应。结论本研究构建了抗氧化基因缺失微生物传感器,实现了对DNA损伤试剂和紫外照射等DNA损伤效应的主动灵敏监测,可为未来空间辐射效应的评价提供一种主动、有效、灵敏的潜在监测方法。

氨磷汀通过调节肠道菌群对急性辐射损伤的防护作用机制

目的探究氨磷汀对急性辐射损伤小鼠的防护作用机制。方法30只C57BL/6J小鼠随机分成正常对照组、模型组和氨磷汀组(150 mg/kg),每组10只。照射前30 min氨磷汀组小鼠腹腔注射氨磷汀,正常对照组和模型组小鼠腹腔注射等体积生理盐水,然后模型组和氨磷汀组小鼠予4 Gy X射线一次性全身照射致急性辐射损伤。检测照射前2 h和照射后第1、4、7、10、14天小鼠外周血中白细胞、血小板和红细胞计数,分析照射后第7天各类白细胞(中性粒细胞、淋巴细胞、单核细胞)的比例变化;采用16S rRNA扩增子测序技术分析照射后第7天小鼠粪便中肠道菌群结构,并与各类白细胞进行相关性分析。结果氨磷汀组小鼠白细胞计数在照射后第1、4、7、10天,血小板计数在照射后第10天,红细胞计数在照射后第1天均显著高于模型组(P<0.05)。与正常对照组比较,模型组小鼠肠道菌群β多样性发生改变,厚壁菌门相对丰度升高,拟杆菌门相对丰度降低;氨磷汀逆转了上述肠道菌群β多样性以及拟杆菌门和厚壁菌门相对丰度的变化。模型组有异芽孢杆菌属、丹毒丝菌纲、丹毒丝菌目和丹毒丝菌科4个差异性物种,其丰度与外周血淋巴细胞比例呈显著负相关(P<0.01),氨磷汀组有小鼠乳杆菌和卷曲乳杆菌2个差异性物种,其丰度与中性粒细胞比例呈显著负相关(P<0.05)。结论氨磷汀可通过维持肠道微生物菌群平衡来减轻辐射造成的急性损伤。

高原强太阳辐射下A^(2)O工艺活性污泥脱氮机制研究

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