CN100577793C - 微生物转化d-果糖制备d-阿洛酮糖的菌种和方法 - Google Patents
微生物转化d-果糖制备d-阿洛酮糖的菌种和方法 Download PDFInfo
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Abstract
微生物转化D-果糖制备D-阿洛酮糖的菌种和方法,属于食品生物技术领域。本发明涉及一株从鱼塘底泥中筛选获得的球形红杆菌(Rhodobactersphaeroides)SK011,保藏编号CCTCC NO:M 207185,及对其培养发酵,并用于转化D-果糖制备D-阿洛酮糖的方法。本发明以SK011作为菌种,采用碳源、氮源、诱导物和无机盐组成的发酵培养基,培养所得菌体进一步处理得到细胞生物催化剂,以D-果糖为底物,生物转化制备D-阿洛酮糖。在优化条件下发酵培养,发酵液或游离细胞或透性化细胞或冻干菌粉或其固定化细胞用于D-果糖转化0.5-48h,转化液中含D-阿洛酮糖2-50g/L。
Description
技术领域
微生物转化D-果糖制备D-阿洛酮糖的菌种和方法,本发明涉及一株筛选获得的球形红杆菌(Rhodobacter sphaeroides)SK011,保藏编号为:CCTCC NO:M207185,及对其培养发酵,并用于转化D-果糖制备D-阿洛酮糖的方法。属于食品生物技术领域。
背景技术
近年来,功能食品成为广大消费者关注的热点,更是广大食品从业者研发的焦点。糖尿病、肥胖和心血管疾病人群的逐年增加和低龄化,使得低热量、具有更多功能营养特性的功能性甜味剂成为关注的热点。
D-阿洛酮糖是一种在自然界中较为稀有的天然己酮糖,属于稀有糖的一种。国际稀有糖协会(ISRS)对稀有糖的定义为“在自然界存在但含量极少的一类单糖及其衍生物”。D-可洛酮糖(D-Psicose)是D-果糖的“差向异构体”。在自然界中少量存在于通过蔗糖水解或者D-葡萄糖异构得到的D-葡萄糖和D-果糖的混合物中,少量出现于甘蔗和甜菜糖蜜加工过程,在小麦、鼠刺属植物和抗生素阿洛酮糖腺苷中也有少量存在。其甜味类似于蔗糖,甜味与D-果糖相当,而热量值只有0.007kcal/g,因此被称为零能量甜味剂。同时D-阿洛酮糖还具有良好的功能特性,如D-阿洛酮糖在消化道仅有少量吸收,且不产生能量,作为一个甜味剂被用作减肥辅助治疗;口服D-阿洛酮糖可抑制肠道α-葡萄糖苷酶活性,防止或减少口服蔗糖和麦芽糖后血糖升高;可抑制肝脏脂肪合成酶活性,减少脂肪沉积;体外实验发现具有神经保护作用,可抑制6-羟基多巴胺诱导的小鼠嗜铬细胞瘤细胞凋亡;与D-葡萄糖和D-果糖相比,具有较强的清除活性氧的能力等。
由于D-阿洛酮糖是一种较为罕见的单糖,其在自然界的含量极低,天然提取分离成本高,不适宜工业化大生产的要求,而化学催化法有许多不利的因素,例如形成许多副产物和化学污染物,而形成的众多副产物又使纯化步骤变得复杂。而生物法制备产物单一,且属于天然产品,符合消费者追求天然产品的消费心理,因此采用生物转化技术生产D-阿洛酮糖,巳成为研究的热点。
用生物转化法制备D-阿洛酮糖的研究已经有10余年的历史,但迄今为止,仅有三种微生物被发现具有生物转化D-果糖制备D-阿洛酮糖的功能,包括Pseudomonas cichorii(Ken Izumori et al.US 5679562,1997;US 5411880,1995)和基因工程菌(Oh D-K,et al.WO 2006129954)中提取得到的酶;以及采用Sinorhizobium sp.(Oh D-K,et al.World Journal of Microbiology and Biotechnology,2007)细胞转化D-果糖制备D-阿洛酮糖。因此,筛选新的微生物菌种进行生物转化制备D-阿洛酮糖成为食品工业从业者的新任务。
发明内容
本发明的目的是筛选出一种能有效生物转化D-果糖为D-阿洛酮糖的新菌株,并提供一种新的生物转化反应生成功能性甜味剂D-阿洛酮糖的方法。
本发明的技术方案:一株转化D-果糖制备D-阿洛酮糖的菌种,其分类命名为球形红杆菌(Rhodobacter sphaeroides)SK011,保藏编号为CCTCC NO:M207185。
用所述球形红杆菌(Rhodobacter sphaeroides)SK011菌株转化D-果糖制备D-阿洛酮糖的方法:
A、菌株的培养:
(1)出发菌株:球形红杆菌(Rhodobacter sphaeroides)SK011;
(2)保藏培养基:葡萄糖营养琼脂培养基;
(3)种子培养基:葡萄糖1-10g/L,玉米浆10-100g/L,尿素1-20g/L,K2HPO4·3H2O 0.1-5g/L,KH2PO40.1-5g/L,MgSO4·7H2O 0.1-5g/L,pH 7.0,去离子水配制;
种子培养条件:用250mL三角瓶装25-70mL种子培养基,按常规方法灭菌、冷却、接种后于30-45℃,150-250r/min摇床培养12-24h作种子培养液;
(4)发酵培养基组成:玉米浆10-100g/L,尿素1-5g/L,K2HPO4·3H2O 0.1-5g/L,KH2PO40.1-5g/L,MgSO4·7H2O 0.1-5g/L,pH 7.0,去离子水配制;
发酵条件:用250mL三角瓶装25-70mL培养基,按常规方法灭菌、冷却、接种后于30-45℃,150-250r/min摇床培养12-24h后添加1.5g/L的D-塔格糖作为诱导物继续培养12-24h;
B、生物转化:
(1)将培养所得到的发酵液进一步处理得到的湿菌体、冻干菌粉、透性化细胞或固定化细胞作为细胞生物催化剂;
(2)将D-果糖按0.1%-75%的比例配制成水溶液作为生物转化底物反应液;
(3)将细胞生物催化剂,加入底物反应液进行转化反应;生物转化反应条件为:底物D-果糖浓度为0.1%-75%,细胞生物催化剂以游离细胞计对底物溶液的用量为10-200g/L;初始pH 5.0-10.0,转化反应温度为20-50℃,150-250r/min摇床培养,转化反应时间0.5-24h;在此条件下所得的转化液用高效液相色谱(HPLC)测定产物量。
C、提纯与精制:将转化反应结束后的反应液用D001型强酸性苯乙烯树脂进行离子交换,去离子水洗涤,再经U20专用树脂纯化,浓缩,结晶,干燥后即得成品D-阿洛酮糖。
一株从鱼塘底泥中筛选获得的微生物菌种SK011,其特征为能耐受高底物浓度,可将D-果糖转化为D-阿洛酮糖,经鉴定该菌株为球形红杆菌Rhodobactersphaeroides SK011(CCTCC NO:M 207185)。
微生物菌株的筛选与鉴定:
本发明从鱼塘底泥中采集土样,接种到富集培养基中进行光照厌氧培养,待培养液明显呈红色,再重复富集培养2次。对富集培养所得菌液采用半固体琼脂培养基梯度稀释厌氧培养,挑选单菌落平板划线得到单菌落后采用D-果糖为单一碳源进行摇瓶发酵,发酵液离心上清采用薄层层析法(TLC法)定性D-阿洛酮糖。将初筛得到的菌株进一步进行复筛,以HPLC法定量测定D-阿洛酮糖浓度,最终筛选出目标菌株SK011。
固定化细胞反复分批转化法是一批转化结束后,过滤,回收固定化细胞,作为下一次转化反应的催化剂,加入新配制的底物继续转化,固定化细胞分批转化试验表明可以连续反复进行多次。
检测D-阿洛酮糖含量的方法:
取反应液离心,上清液微孔滤膜过滤(0.22μm),滤液上HPLC分析。HPLC条件:Waters2410色谱柱:Sugarpak1,6.5mm id×300mm钙型阳离子交换柱,流动相:纯水,检测器:示差折光检测器,柱温:85℃,流速:0.4mL/min,进样量:10μL,D-阿洛酮糖标样浓度:0.5%。
本发明的有益效果:本发明以SK011作为菌种,采用碳源、氮源、诱导物和无机盐组成的发酵培养基,培养所得菌体进一步处理得到细胞生物催化剂,以D-果糖为底物,生物转化制备D-阿洛酮糖。在优化条件下发酵培养,发酵液或游离细胞或透性化细胞或冻干菌粉或其固定化细胞用于D-果糖转化0.5-48h,转化液中含D-阿洛酮糖2-50g/L。筛选出的新的微生物菌种SK011进行生物转化制备D-阿洛酮糖比国外报道的野生菌转化制备D-阿洛酮糖的转化率为高。
生物材料样品保藏
一种用于微生物转化D-果糖制备D-阿洛酮糖的菌株,分类命名为球形红杆菌(Rhodobacter sphaeroides)SK011,已保藏于中国典型培养物保藏中心,简称CCTCC,其保藏编号为CCTCC NO:M 207185,保藏日期:2007年11月26日。
具体实施方式
以下是SK011进行生物转化D-果糖制备D-阿洛酮糖的实施例,说明本发明的方法,但本发明并不限于所列出的几个实例。
实施例1
用SK011进行培养发酵,斜面培养基为葡萄糖营养琼脂培养基。种子培养基组成为葡萄糖3g/L;玉米浆20g/L;尿素10g/L;K2HPO4.3H2O 0.8g/L;KH2PO42.5g/L,MgSO4.7H2O 0.9g/L;pH 7.0;种子培养基培养条件:用250mL三角瓶装50mL培养基,按常规方法灭菌、冷却、接种后于30℃,180r/min摇床培养24h作为种子培养液。发酵培养基组成为:玉米浆30g/L,尿素2g/L,K2HPO4.3H2O 3g/L,KH2PO43g/L,MgSO4.7H2O 1g/L,pH 7.0,去离子水配制;发酵条件:用250mL三角瓶装45mL培养基,按常规方法灭菌、冷却、接种后于33℃,180r/min摇床培养12h后添加1.5g/L的D-塔格糖作为诱导物继续培养24h,最终获得细胞干重为2g/L的发酵液。
将50mL发酵液经5000g,4℃,离心10min得到湿菌体量0.5g,在50mL三角瓶中加入10mL 1%D-果糖溶液,初始pH值5.0,37℃,180r/min振荡转化24小时,测得反应液中D-阿洛酮糖浓度为4g/L。
实施例2
按实施例1方法用SK011进行培养发酵,得到的湿菌体0.8g,加入5%的十六烷基三甲基溴化铵对细胞进行透性化处理,室温处理20min后用生理盐水洗细胞2次后,在50mL三角瓶中加入10mL 10%D-果糖溶液,初始pH值8.0,25℃,180r/min振荡转化12小时,测得反应液中D-阿洛酮糖浓度为6g/L。
实施例3
按实施例1方法用SK011进行培养发酵,得到的湿菌体9g,加入1%甲苯对细胞进行透性化处理,室温处理20min后用生理盐水洗细胞2次后,在50mL三角瓶中加入10mL 50%D-果糖溶液,初始pH值10.0,45℃,180r/min振荡转化1小时,测得反应液中D-阿洛酮糖浓度为46g/L。
实施例4
按实施例1方法用SK011进行培养发酵,得到的湿菌体0.8g,用8mL生理盐水调成10%菌悬液;另用0.9g藻酸钠,20mL生理盐水,配制成4.5%浓度的海藻酸钠溶液,煮沸溶解,冷却至45℃左右;与菌悬液混合搅拌均匀,用胶头滴管滴入100mL 0.1M的CaCl2溶液中,于4℃下浸泡硬化4h后即为固定化细胞用于生物转化。按实施例2方式用8g固定化细胞与0.8g湿菌体细胞对照进行转化,反复分批转化结果如表1所示。
表1固定化细胞反复分批转化结果
Claims (2)
1、一株转化D-果糖制备D-阿洛酮糖的菌种,其分类命名为球形红杆菌(Rhodobacter sphaeroides)SK011,保藏编号为CCTCC NO:M 207185。
2、用权利要求1所述球形红杆菌(Rhodobacter sphaeroides)SK011菌株转化D-果糖制备D-阿洛酮糖的方法,其特征是
A、菌株的培养:
(1)出发菌株:球形红杆菌(Rhodobacter sphaeroides)SK011;
(2)保藏培养基:葡萄糖营养琼脂培养基;
(3)种子培养基:葡萄糖1-10g/L,玉米浆10-100g/L,尿素1-20g/L,K2HPO4·3H2O 0.1-5g/L,KH2PO4 0.1-5g/L,MgSO4·7H2O 0.1-5g/L,pH 7.0,去离子水配制;
种子培养条件:用250mL三角瓶装25-70mL种子培养基,按常规方法灭菌、冷却、接种后于30-45℃,150-250r/min摇床培养12-24h作种子培养液;
(4)发酵培养基组成:玉米浆10-100g/L,尿素1-5g/L,K2HPO4·3H2O 0.1-5g/L,KH2PO40.1-5g/L,MgSO4·7H2O 0.1-5g/L,pH 7.0,去离子水配制;
发酵条件:用250mL三角瓶装25-70mL培养基,按常规方法灭菌、冷却、接种后于30-45℃,150-250r/min摇床培养12-24h后添加1.5g/L的D-塔格糖作为诱导物继续培养12-24h;
B、生物转化:
(1)将培养所得到的发酵液进一步处理得到的湿菌体、冻干菌粉、透性化细胞或固定化细胞作为细胞生物催化剂;
(2)将D-果糖按0.1%-75%的比例配制成水溶液作为生物转化底物反应液;
(3)将细胞生物催化剂,加入底物反应液进行转化反应;生物转化反应条件为:底物D-果糖浓度为0.1%-75%,细胞生物催化剂以游离细胞计对底物溶液的用量为10-200g/L;初始pH 5.0-10.0,转化反应温度为20-50℃,150-250r/min摇床培养,转化反应时间0.5-24h;
C、提纯与精制:将转化反应结束后的反应液用D001型强酸性苯乙烯树脂进行离子交换,去离子水洗涤,再经U20专用树脂纯化,浓缩,结晶,干燥后即得成品D-阿洛酮糖。
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